US20200054669A1 - Compositions for and methods of treating acid-base disorders - Google Patents

Compositions for and methods of treating acid-base disorders Download PDF

Info

Publication number
US20200054669A1
US20200054669A1 US16/099,045 US201716099045A US2020054669A1 US 20200054669 A1 US20200054669 A1 US 20200054669A1 US 201716099045 A US201716099045 A US 201716099045A US 2020054669 A1 US2020054669 A1 US 2020054669A1
Authority
US
United States
Prior art keywords
meq
serum bicarbonate
way
further example
bicarbonate value
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Abandoned
Application number
US16/099,045
Other languages
English (en)
Inventor
Gerrit Klaerner
Eric F. CONNOR
Randi K. GBUR
Matthew J. KADE
Paul H. KIERSTEAD
Jerry M. Buysse
Michael J. Cope
Kalpesh N. BIYANI
Son H. Nguyen
Scott M. Tabakman
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Renosis Inc
Original Assignee
Tricida Inc
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Tricida Inc filed Critical Tricida Inc
Priority to US16/099,045 priority Critical patent/US20200054669A1/en
Assigned to TRICIDA, INC. reassignment TRICIDA, INC. ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS). Assignors: KLAERNER, GERRIT, BIYANI, KALPESH N., KIERSTEAD, PAUL H., NGUYEN, SON H., TABAKMAN, SCOTT M., BUYSSE, JERRY M., KADE, MATTHEW J., GBUR, RANDI K., CONNOR, ERIC F., COPE, MICHAEL J.
Publication of US20200054669A1 publication Critical patent/US20200054669A1/en
Assigned to RENOSIS, INC. reassignment RENOSIS, INC. ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS). Assignors: TRICIDA, INC.
Abandoned legal-status Critical Current

Links

Images

Classifications

    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K31/00Medicinal preparations containing organic active ingredients
    • A61K31/13Amines
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K31/00Medicinal preparations containing organic active ingredients
    • A61K31/74Synthetic polymeric materials
    • A61K31/785Polymers containing nitrogen
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K33/00Medicinal preparations containing inorganic active ingredients
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/0012Galenical forms characterised by the site of application
    • A61K9/0053Mouth and digestive tract, i.e. intraoral and peroral administration
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/10Dispersions; Emulsions
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/14Particulate form, e.g. powders, Processes for size reducing of pure drugs or the resulting products, Pure drug nanoparticles
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/20Pills, tablets, discs, rods
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P13/00Drugs for disorders of the urinary system
    • A61P13/12Drugs for disorders of the urinary system of the kidneys
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P3/00Drugs for disorders of the metabolism
    • A61P3/12Drugs for disorders of the metabolism for electrolyte homeostasis
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P43/00Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08FMACROMOLECULAR COMPOUNDS OBTAINED BY REACTIONS ONLY INVOLVING CARBON-TO-CARBON UNSATURATED BONDS
    • C08F8/00Chemical modification by after-treatment
    • C08F8/02Alkylation
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08FMACROMOLECULAR COMPOUNDS OBTAINED BY REACTIONS ONLY INVOLVING CARBON-TO-CARBON UNSATURATED BONDS
    • C08F226/00Copolymers of compounds having one or more unsaturated aliphatic radicals, each having only one carbon-to-carbon double bond, and at least one being terminated by a single or double bond to nitrogen or by a heterocyclic ring containing nitrogen
    • C08F226/02Copolymers of compounds having one or more unsaturated aliphatic radicals, each having only one carbon-to-carbon double bond, and at least one being terminated by a single or double bond to nitrogen or by a heterocyclic ring containing nitrogen by a single or double bond to nitrogen
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08FMACROMOLECULAR COMPOUNDS OBTAINED BY REACTIONS ONLY INVOLVING CARBON-TO-CARBON UNSATURATED BONDS
    • C08F226/00Copolymers of compounds having one or more unsaturated aliphatic radicals, each having only one carbon-to-carbon double bond, and at least one being terminated by a single or double bond to nitrogen or by a heterocyclic ring containing nitrogen
    • C08F226/02Copolymers of compounds having one or more unsaturated aliphatic radicals, each having only one carbon-to-carbon double bond, and at least one being terminated by a single or double bond to nitrogen or by a heterocyclic ring containing nitrogen by a single or double bond to nitrogen
    • C08F226/04Diallylamine

Definitions

  • the present invention generally relates to methods of treating acid-base disorders that may be used, for example, in the treatment of metabolic acidosis.
  • Metabolic acidosis is the result of metabolic and dietary processes that in various disease states create a condition in which non-volatile acids accumulate in the body, causing a net addition of protons (H + ) or the loss of bicarbonate (HCO 3 ⁇ ). Metabolic acidosis occurs when the body accumulates acid from metabolic and dietary processes and the excess acid is not completely removed from the body by the kidneys. Chronic kidney disease is often accompanied by metabolic acidosis due to the reduced to capacity of the kidney to excrete hydrogen ions secondary to an inability to reclaim filtered bicarbonate (HCO 3 ⁇ ), synthesize ammonia (ammoniagenesis), and excrete titratable acids.
  • Clinical practice guidelines recommend initiation of alkali therapy in patients with non-dialysis-dependent chronic kidney disease (CKD) when the serum bicarbonate level is ⁇ 22 mEq/L to prevent or treat complications of metabolic acidosis.
  • CKD non-dialysis-dependent chronic kidney disease
  • Clinical practice guidelines for nutrition in chronic renal failure K/DOQI, National Kidney Foundation, Am. J. Kidney Dis. 2000; 35:S1-140; Raphael, K L, Zhang, Y, Wei, G, et al. 2013, Serum bicarbonate and mortality in adults in NHANES III, Nephrol. Dial. Transplant 28: 1207-1213).
  • These complications include malnutrition and growth retardation in children, exacerbation of bone disease, increased muscle degradation, reduced albumin synthesis, and increased inflammation.
  • Metabolic acidosis regardless of etiology, lowers extracellular fluid bicarbonate and, thus, decreases extracellular pH.
  • the relationship between serum pH and serum bicarbonate is described by the Henderson-Hasselbalch equation
  • pH pK′+log [HCO 3 ⁇ ]/[(0.03 ⁇ PaCO 2 )]
  • VBG Venous blood gas
  • measurement of venous plasma bicarbonate or total carbon dioxide [tCO 2 ]
  • arterial plasma bicarbonate or total carbon dioxide [tCO 2 ]
  • serum electrolytes Cl ⁇ , K + , and Na + serum electrolytes Cl ⁇ , K + , and Na +
  • measurement of venous plasma or serum electrolytes includes an estimation of the tCO 2 . This measurement reflects the sum of circulating CO 2 [i.e., the total CO 2 represented by bicarbonate (HCO 3 ⁇ ), carbonic acid, (H 2 CO 3 ) and dissolved CO 2 (0.03 ⁇ PCO 2 )].
  • tCO 2 can also be related to HCO 3 ⁇ by using a simplified and standardized form of the Henderson-Hasselbalch equation: tCO 2 ⁇ HCO 3 +0.03 PCO 2 , where PCO 2 is the measured partial pressure of CO 2 . Since HCO 3 ⁇ concentration is greater than 90% of the tCO 2 , and there are small amounts of H 2 CO 3 , then venous tCO 2 is often used as a reasonable approximation of the venous HCO 3 ⁇ concentration in the blood. Especially during chronic kidney disease, an abnormal plasma HCO 3 ⁇ value ⁇ 22 mEq/L generally indicates metabolic acidosis.
  • Calculation of the anion gap [defined as the serum Na + — (Cl ⁇ +HCO 3 ⁇ )] is an important aspect of the diagnosis of metabolic acidosis.
  • Metabolic acidosis may be present with a normal or an elevated anion gap.
  • an elevated anion gap commonly signifies the presence of metabolic acidosis, regardless of the change in serum HCO 3 ⁇ .
  • An anion gap greater than 20 mEq/L normal anion gap is 8 to 12 mEq/L is a typical feature of metabolic acidosis.
  • Arterial blood gases are used to identify the type of an acid-base disorder and to determine if there are mixed disturbances. In general, the result of arterial blood gas measures should be coordinated with history, physical exam and the routine laboratory data listed above.
  • An arterial blood gas measures the arterial carbon dioxide tension (P a CO 2 ), acidity (pH), and the oxygen tension (P a O 2 ).
  • the HCO 3 ⁇ concentration is calculated from the pH and the PaCO 2 . Hallmarks of metabolic acidosis are a pH ⁇ 7.35, P a CO 2 ⁇ 35 mm Hg and HCO 3 ⁇ ⁇ 22 mEq/L.
  • Acid-base disturbance are first classified as respiratory or metabolic. Respiratory disturbances are those caused by abnormal pulmonary elimination of CO 2 , producing an excess (acidosis) or deficit (alkalosis) of CO 2 (carbon dioxide) in the extracellular fluid. In respiratory acid-base disorders, changes in serum bicarbonate (HCO 3 ⁇ ) are initially a direct consequence of the change in PCO 2 with a greater increase in PCO 2 resulting in an increase in HCO 3 ⁇ .
  • HCO 3 ⁇ serum bicarbonate
  • Metabolic disturbances are those caused by excessive intake of, or metabolic production or losses of, nonvolatile acids or bases in the extracellular fluid. These changes are reflected by changes in the concentration of bicarbonate anion (HCO 3 ⁇ ) in the blood; adaptation in this case involves both buffering (immediate), respiratory (hours to days) and renal (days) mechanisms.
  • HCO 3 ⁇ bicarbonate anion
  • the overall hydrogen ion concentration in the blood is defined by the ratio of two quantities, the serum HCO 3 ⁇ content (regulated by the kidneys) and the PCO 2 content (regulated by the lungs) and is expressed as follows:
  • Bicarbonate (HCO 3 ⁇ ) is an anion that acts to buffer against pH disturbances in the body, and normal levels of plasma bicarbonate range from 22-26 mEq/L (Szerlip H M: Metabolic Acidosis, 2005, in Greenberg A, Cheung A K (eds) Primer on Kidney Diseases, National Kidney Foundation, Philadelphia, Elsevier-Saunders, pp. 74-89). Acidosis is the process which causes a reduction in blood pH (acidemia) and reflects the accumulation of hydrogen ion (H + ) and its consequent buffering by bicarbonate ion (HCO 3 ⁇ ) resulting in a decrease in serum bicarbonate. Metabolic acidosis can be represented as follows:
  • nonvolatile acids ⁇ 50-100 mEq/day are produced by the metabolism of sulfate- and phosphate-containing amino acids and nucleic acids. Additional nonvolatile acids (lactic acid, butyric acid, acetic acid, other organic acids) arise from the incomplete oxidation of fats and carbohydrates, and from carbohydrate metabolism in the colon, where bacteria residing in the colon lumen convert the substrates into small organic acids that are then absorbed into the bloodstream. The impact of short chain fatty acids on acidosis is somewhat minimized by anabolism, for example into long-chain fatty acids, or catabolism to water and CO 2 .
  • the kidneys maintain pH balance in the blood through two mechanisms: reclaiming filtered HCO 3 ⁇ to prevent overall bicarbonate depletion and the elimination of nonvolatile acids in the urine. Both mechanisms are necessary to prevent bicarbonate depletion and acidosis.
  • the kidneys reclaim HCO 3 ⁇ that is filtered by the glomerulus. This reclamation occurs in the proximal tubule and accounts for ⁇ 4500 mEq/day of reclaimed HCO 3 ⁇ . This mechanism prevents HCO 3 ⁇ from being lost in the urine, thus preventing metabolic acidosis.
  • the kidneys eliminate enough H + to equal the daily nonvolatile acid production through metabolism and oxidation of protein, fats and carbohydrates. Elimination of this acid load is accomplished by two distinct routes in the kidney, comprising active secretion of H + ion and ammoniagenesis. The net result of these two interconnected processes is the elimination of the 50-100 mEq/day of nonvolatile acid generated by normal metabolism.
  • Sodium bicarbonate NaHCO 3
  • NaHCO 3 is the agent most commonly used to correct metabolic acidosis.
  • NaHCO 3 can be administered intravenously to raise the serum HCO 3 ⁇ level adequately to increase the pH to greater than 7.20. Further correction depends on the individual situation and may not be indicated if the underlying process is treatable or the patient is asymptomatic. This is especially true in certain forms of metabolic acidosis. For example, in high-anion gap (AG) acidosis secondary to accumulation of organic acids, lactic acid, and ketones, the cognate anions are eventually metabolized to HCO 3 ⁇ .
  • AG high-anion gap
  • the serum pH corrects; thus, caution should be exercised in these patients when providing alkali to raise the pH much higher than 7.20, to prevent an increase in bicarbonate above the normal range (>26 mEq/L).
  • Citrate is an appropriate alkali therapy to be given orally or IV, either as the potassium or sodium salt, as it is metabolized by the liver and results in the formation of three moles of bicarbonate for each mole of citrate.
  • Potassium citrate administered IV should be used cautiously in the presence of renal impairment and closely monitored to avoid hyperkalemia.
  • Intravenous sodium bicarbonate (NaHCO 3 ) solution can be administered if the metabolic acidosis is severe or if correction is unlikely to occur without exogenous alkali administration.
  • Oral alkali administration is the preferred route of therapy in persons with chronic metabolic acidosis.
  • the most common alkali forms for oral therapy include NaHCO 3 tablets where 1 g of NaHCO 3 is equal to 11.9 mEq of HCO 3 ⁇ .
  • the oral form of NaHCO 3 is not approved for medical use and the package insert of the intravenous sodium bicarbonate solution includes the following contraindications, warnings and precautions (Hospira label for NDC 0409-3486-16):
  • Acid-base disorders are common in chronic kidney disease and heart failure patients.
  • Chronic kidney disease CKD
  • CKD progressively impairs renal excretion of the approximately 1 mmol/kg body weight of hydrogen ions generated in healthy adults (Yaqoob, M M. 2010, Acidosis and progression of chronic kidney disease, Curr. Opin. Nephrol. Hyperten. 19:489-492).
  • Metabolic acidosis resulting from the accumulation of acid (H + ) or depletion of base (HCO 3 ⁇ ) in the body, is a common complication of patients with CKD, particularly when the glomerular filtration rate (GFR, a measure of renal function) falls below 30 ml/min/1.73 m 2 .
  • GFR glomerular filtration rate
  • Metabolic acidosis has profound long term effects on protein and muscle metabolism, bone turnover and the development of renal osteodystrophy.
  • metabolic acidosis influences a variety of paracrine and endocrine functions, again with long term consequences such as increased inflammatory mediators, reduced leptin, insulin resistance, and increased corticosteroid and parathyroid hormone production (Mitch W E, 1997, Influence of metabolic acidosis on nutrition, Am. J. Kidney Dis. 29:46-48).
  • CKD patients of moderate degree first develop hyperchloremic acidosis with a normal anion gap due to the inability to reclaim filtered bicarbonate and excrete proton and ammonium cations. As they progress toward the advanced stages of CKD the anion gap increases, reflective of the continuing degradation of the kidney's ability to excrete the anions that were associated with the unexcreted protons. Serum bicarbonate in these patients rarely goes below 15 mmol/L with a maximum elevated anion gap of approximately 20 mmol/L.
  • kidney, heart failure, diabetes and hypertensive guidelines strictly limit sodium intake in these patients to less than 1.5 g or 65 mEq per day (HFSA 2010 guidelines, Lindenfeld 2010, J Cardiac Failure V16 No 6 P 475).
  • Chronic anti-hypertensive therapies often induce sodium excretion (diuretics) or modify the kidney's ability to excrete sodium and water (such as, for example, Renin Angiotensin Aldosterone System inhibiting “RAASi” drugs).
  • RAASi drugs induce life-threatening hyperkalemia as they inhibit renal potassium excretion.
  • metabolic acidosis patients with amounts of sodium-containing base that often exceed the total daily recommended sodium intake is not a reasonable practice.
  • oral sodium bicarbonate is not commonly prescribed chronically in these diabetic nephropathy patients.
  • Potassium bicarbonate is also not acceptable as patients with CKD are unable to readily excrete potassium, leading to severe hyperkalemia.
  • Stage 5 End Stage CKD (GFR ⁇ 15 mL/min/1.73 m 2 ).
  • the average dose of bicarbonate in this study was 1.82 g/day, which provides 22 mEq of bicarbonate per day.
  • the primary end points were rate of CrCl decline, the proportion of patients with rapid decline of CrCl (>3 ml/min per 1.73 m 2 /yr), and end-stage renal disease (“ESRD”) (CrCl ⁇ 10 ml/min).
  • ESRD end-stage renal disease
  • Hyperphosphatemia is a common co-morbidity in patients with CKD, particularly in those with advanced or end-stage renal disease.
  • Sevelamer hydrochloride is a commonly used ion-exchange resin that reduces serum phosphate concentration.
  • reported drawbacks of this agent include metabolic acidosis apparently due to the net absorption of HCl in the process of binding phosphate in the small intestine.
  • Several studies in patients with CKD and hyperphosphatemia who received hemodialysis or peritoneal dialysis found decreases in serum bicarbonate concentrations with the use of sevelamer hydrochloride (Brezina, 2004 Kidney Int. V66 S90 (2004) S39-S45; Fan, 2009 Nephrol Dial Transplant (2009) 24:3794).
  • the following is a useful guide for one method for treating metabolic acidosis (without wishing to be bound by theory).
  • a HCO 3 ⁇ enters the systemic circulation and raises the serum bicarbonate concentration.
  • the initial binding of gastric H + to a nonabsorbable composition as described herein results in HCO 3 ⁇ entering the systemic circulation and raising the serum bicarbonate concentration.
  • the binding of Cl ⁇ the nonabsorbable composition prevents subsequent exchange of luminal Cl ⁇ for HCO 3 ⁇ which would counteract the initial rise in HCO 3 + .
  • the analogous clinical situation to administering the composition is vomiting.
  • composition is essentially causing the loss of gastric HCl as in vomiting. If a person vomits they lose gastric HCl and have an increase in serum bicarbonate. The increase in serum bicarbonate persists only if they are not given a lot of oral Cl ⁇ , for example as NaCl, which would allow subsequent exchange of intestinal Cl ⁇ for HCO 3 ⁇ and dissipate the increase in serum bicarbonate concentration.
  • oral Cl ⁇ for example as NaCl
  • a method of treating an individual afflicted with a chronic acid/base disorder characterized by a baseline serum bicarbonate value of less than 22 mEq/l comprises oral administration of a pharmaceutical composition comprising a nonabsorbable composition having the capacity to bind a target species selected from the group consisting of protons, a conjugate base of a strong acid, and a strong acid as it transits the digestive system.
  • Another aspect of the present disclosure is a method of treating an individual afflicted with an acid-base disorder characterized by a baseline serum bicarbonate value of less than 22 mEq/l, the method comprising oral administration of a daily dose of a pharmaceutical composition having the capacity to remove at least 5 meq of a target species as it transits the digestive system to achieve a clinically significant increase in the serum bicarbonate value of at least 1 mEq/l from baseline within a treatment period not greater than 1 month.
  • the target species is selected from the group consisting of protons, strong acids, and conjugate bases of strong acids.
  • compositions for use in a method of treating metabolic acidosis in an adult human patient wherein in said treatment 0.1-12 g of said composition is administered to the patient per day, said composition being a nonabsorbable composition having the capacity to remove protons from the patient, wherein the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 2.5 mEq/g in a Simulated Small Intestine Inorganic Buffer (“SIB”) assay.
  • SIB Simulated Small Intestine Inorganic Buffer
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • compositions for use in a method of treating metabolic acidosis in an adult human patient said patient having a serum bicarbonate level of less than 20 mEq/L prior to treatment, said composition being a nonabsorbable composition having the capacity to remove protons from the patient.
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • SIB Simulated to Small Intestine Inorganic Buffer
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • SIB Simulated Small Intestine Inorganic Buffer
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • the orally administered nonabsorbable composition comprises cations (such as Na + , K + , Mg 2+ , Ca 2+ Li + , or a combination thereof) that are exchanged for protons as the nonabsorbable composition transits the digestive system, and the protons are then excreted from the body along with the nonabsorbable composition upon defecation.
  • the net effect is reduction in protons in the body, in exchange for an increase in one or more cations.
  • the pharmaceutical composition may also optionally comprise a pharmaceutically acceptable carrier, diluent or excipient, or a combination thereof that does not significantly interfere with the proton-binding characteristics of the nonabsorbable composition in vivo.
  • the pharmaceutical composition may also comprise an additional therapeutic agent.
  • the orally administered nonabsorbable composition comprises anions that are exchanged for chloride ions and if the anion comprised by the orally administered nonabsorbable composition is a stronger base (e.g., OH ⁇ ) than the removed base (e.g., Cl + , HSO 4 ⁇ , or SO 4 2 ⁇ ), the net effect is the removal of a strong acid from the body (e.g., HCl or H 2 SO 4 ) in exchange for a weak acid (e.g., H 2 O).
  • a strong acid from the body e.g., HCl or H 2 SO 4
  • a weak acid e.g., H 2 O
  • the pharmaceutical composition may also optionally comprise a pharmaceutically acceptable carrier, diluent or excipient, or a combination thereof that does not significantly interfere with the chloride-binding characteristics of the nonabsorbable composition in vivo.
  • the pharmaceutical composition may also comprise an additional therapeutic agent.
  • the orally administered nonabsorbable composition is a neutral composition having the capacity to bind and remove a strong acid, such as HCl or H 2 SO 4 , from the body upon oral administration.
  • the nonabsorbable composition may, but does not necessarily, introduce (i.e., by ion exchange) counterbalancing cations or anions in the process of removing the acid.
  • binding of both ionic species of HCl H + and Cl ⁇
  • binding of both ionic species of HCl may be achieved through favorable surface energy of the bulk material, which can include hydrogen bonding and other interactions as well as ionic interactions.
  • Complexation of HCl can occur on functional groups that are dehydrated and upon administration in an acidic aqueous medium, result in the hydrochloride salt of the functional group.
  • a method of treating an individual afflicted with a chronic acid/base disorder comprising oral administration of a pharmaceutical composition containing a nonabsorbable composition having the capacity to bind protons and chloride ions as it transits the digestive system and remove the bound protons and chloride ions from the individual's digestive system via defecation.
  • the pharmaceutical composition may also optionally comprise a pharmaceutically acceptable carrier, diluent or excipient, or a combination thereof that does not significantly interfere with the chloride-binding characteristics of the nonabsorbable composition in vivo.
  • the pharmaceutical composition may also comprise an additional therapeutic agent.
  • any of the methods of treating an individual afflicted with an acid-base disorder disclosed in this application comprise: i) the individual having a diet regimen, or ii) the method including, specifying, prescribing or recommending a diet regimen.
  • said diet regimen is an alkaline diet regimen.
  • said diet regimen is a conventional low-protein diet regimen ( ⁇ 0.6 g/kg per day).
  • said diet regimen is a very low-protein diet regimen (0.3-0.4 g/kg per day).
  • said diet regimen is a vegetarian diet regimen.
  • said said diet regimen is a vegetarian diet regimen supplemented with either essential amino acids or a mixture of essential amino acids and nitrogen-free ketoanalogues (keto diet regimen).
  • said diet regimen is ketoanalogue-supplemented vegetarian very low-protein diet. In one embodiment, said diet regimen is a vegan diet regimen. In one embodiment, said diet regimen is a casein diet regimen. In one embodiment, said diet regimen is an adenine-containing diet regimen. In one embodiment, said diet regimen comprises one or more base-producing vegetables (e.g. carrots, cauliflower, eggplant, lettuce, potatoes, spinach, tomatoes, or zucchini, or a combination thereof). In one embodiment, said diet regimen comprises one or more base-producing fruits (e.g. apple, apricot, oranges, peaches, pears, raisins, or strawberries, or a combination thereof). In one embodiment, said diet regimen does not comprise acid-producing meat.
  • said diet regimen does not comprise acid-producing meat.
  • the diet comenses one year before administering the nonabsorbable composition. In another embodiment the diet comenses six months before administering the nonabsorbable composition. In another embodiment the diet comenses one month before administering the nonabsorbable composition. In another embodiment the diet regimen comenses when the administering of the nonabsorbable composition comenses. In another embodiment the diet comenses one month after administering the nonabsorbable composition. In another embodiment the diet comenses six months after administering the nonabsorbable composition. In another embodiment the diet comenses one year after administering the nonabsorbable composition.
  • Gameata et al. assessed the effects of a ketoanalogue-supplemented vegetarian very low protein diet (0.3 g/kg/day) in diet-compliant patients to those of a usual mixed-source low protein diet (0.6 g/kg/day).
  • Baseline serum bicarbonate was similar in the two treatment groups (16.7-16.8 mEq/L), however the end of study serum bicarbonate value was significantly higher in the vegetarian very low protein diet group than the usual mixed-source low protein diet group.
  • Efficacy of the vegetarian very low protein diet to reduce incidence of renal events was most noted in patients with initial eGFR ⁇ 20 mL/min ⁇ 1.73 m 2 .
  • the nonabsorbable composition binds chloride ions
  • the nonabsorbable composition selectively bind chloride ions relative to other physiologically significant competing anions such as bicarbonate equivalent anions, phosphate anions, and the conjugate bases of bile and fatty acids that are present in the GI tract.
  • the nonabsorbable composition remove more chloride ions than any other competing anion in the GI tract.
  • the nonabsorbable composition binds protons
  • the nonabsorbable composition bind protons without delivering sodium, potassium, calcium, magnesium, and/or other electrolytes in exchange for the protons in an amount that is physiologically detrimental.
  • treatment with the nonabsorbable composition will not significantly contribute to edema, hypertension, hyperkalemia, hypercalcemia or a similar disorder associated with an elevated load of sodium, potassium, calcium or other electrolyte.
  • the nonabsorbable composition binds protons
  • the nonabsorbable composition bind protons without removing an amount of sodium, potassium, calcium, magnesium and/or other electrolytes along with the protons.
  • treatment with the nonabsorbable composition will not significantly contribute to hypotension, hypokalemia, hypocalcemia or other disorder associated with a depressed serum concentration of sodium, potassium, calcium, magnesium or other electrolyte.
  • the polymers preferably bind and maintain their ability to bind proton and anions at the physiological conditions found along the gastrointestinal (GI) lumen. These conditions can change according to dietary intake (see, for example, Fordtran J, Locklear T. Ionic constituents and osmolality of gastric and small-intestinal fluids after eating. Digest Dis Sci. 1966; 11(7):503-21) and location along the GI tract (Binder, H et al. Chapters 41-45 in “Medical Physiology”, 2nd Edition, Elsevier [2011]. Boron and Boulpaep [Ed.]). Rapid binding of proton and chloride in the stomach and small intestine is desirable.
  • GI gastrointestinal
  • the polymers also preferably have a pK such that the majority of amines are protonated under the various pH and electrolyte conditions encountered along the GI tract and are thereby capable of removing proton, along with an appropriate counter anion (preferably chloride), from the body into the feces.
  • the stomach is an abundant source of HCl, and the stomach is the first site of potential HCl binding (after the mouth), and since residence time in the stomach is short (gastric residence half-life of approximately 90 minutes), compared to the rest of the GI tract (small intestine transit time of approximately 4 hours; whole gut transit time of 2-3 days; Read, N W et al. Gastroenterology [1980] 79:1276), it is desirable for the polymer of the present disclosure to demonstrate rapid kinetics of proton and chloride binding in the lumen of this organ, as well as in in vitro conditions designed to mimic the stomach lumen (e.g. SGF).
  • SGF stomach lumen
  • Phosphate is a potential interfering anion for chloride binding in the stomach and small intestine, where phosphate is mostly absorbed (Cross, H S et al Miner Electrolyte Metab [1990] 16:115-24). Therefore rapid and preferential binding of chloride over phosphate is desirable in the small intestine and in in vitro conditions designed to mimic the small intestine lumen (e.g. SIB).
  • FIG. 1A-1C is a flow chart schematically depicting the mechanism of action of the polymer when passing through the gastrointestinal tract of an individual from oral ingestion/stomach ( FIG. 1A ), to the upper GI tract ( FIG. 1B ) to the lower GI tract/colon ( FIG. 1C ).
  • FIG. 2 is a graph of the effect of TRC101 on serum bicarbonate in a rat model of adenine-induced nephropathy and metabolic acidosis in Part 1 of the study described in Example 1.
  • FIGS. 3A, 3B and 3C are graphs of the effect of TRC101 on fecal excretion of chloride ( FIG. 3A ), sulfate ( FIG. 3B ), and phosphate ( FIG. 3C ) in a rat model of adenine-induced nephropathy and metabolic acidosis in Part 1 of the study described in Example 1.
  • FIG. 4 is a graph of the effect of TRC101 on serum bicarbonate in a rat model of adenine-induced nephropathy and metabolic acidosis in Part 2 of the study described in Example 1.
  • FIGS. 5A, 5B and 5C are graphs of the effect of TRC101 on fecal excretion of chloride ( FIG. 5A ), sulfate ( FIG. 5B ), and phosphate ( FIG. 5C ) in a rat model of adenine-induced nephropathy and metabolic acidosis in Part 2 of the study described in Example 1.
  • FIGS. 6A, 6B and 6C are graphs of the in vivo chloride ( FIG. 6A ), sulfate ( FIG. 6B ) and phosphate ( FIG. 6C ) binding capacities of test compound and bixalomer in a pig with normal renal function in the study described in Example 2.
  • FIG. 7 is a line graph showing the mean change in serum bicarbonate (SBC) from baseline (BL) and standard error (SE) by treatment group over time in a human study as described more fully in Example 3 (Part 1).
  • SBC serum bicarbonate
  • SE standard error
  • FIG. 8 is a bar graph showing the least squares mean (LS Mean) change from baseline (CFB) to end of treatment in serum bicarbonate (SBC) by treatment group in a human study as described more fully in Example 3 (Part 1).
  • LS Mean least squares mean
  • SBC serum bicarbonate
  • SE standard error
  • FIG. 10 is a line graph showing the mean change in serum bicarbonate (SBC) and standard error (SE) for the four TRC101 active arms and the two placebo arms (pooled) of the study described more fully in Example 3 (Parts 1 and 2).
  • SBC serum bicarbonate
  • SE standard error
  • FIG. 11 is a bar graph showing the least squares mean (LS Mean) change from baseline (CFB) in serum bicarbonate (SBC) by treatment group over time for the four TRC101 active arms and the two placebo arms (pooled) of the study described more fully in Example 3 (Parts 1 and 2).
  • LS Mean least squares mean
  • CBC serum bicarbonate
  • SBC serum bicarbonate
  • SE standard error
  • FIGS. 13A, 13B, 13C and 13D are graphs showing the changes in serum bicarbonate ( FIG. 13A ), serum chloride ( FIG. 13B ), serum sodium ( FIG. 13C ) and serum potassium ( FIG. 13D ) for the four TRC101 active arms (combined) vs the two placebo arms (pooled) over time for the study described more fully in Example 3 (Parts 1 and 2).
  • FIG. 14 is a graph showing the changes in the calculated anion gap for the four TRC101 active arms (combined) vs the two placebo arms (pooled) over time for the study described more fully in Example 3 (Parts 1 and 2).
  • absorption capacity as used herein in connection with a polymer and a swelling agent (or in the case of a mixture of swelling agents, the mixture of swelling agents) is the amount of the swelling agent (or such mixture) absorbed during a period of at least 16 hours at room temperature by a given amount of a dry polymer (e.g., in the form of a dry bead) immersed in an excess amount of the swelling agent (or such mixture).
  • acrylamide denotes a moiety having the structural formula H 2 C ⁇ CH—C(O)NR—*, where * denotes the point of attachment of the moiety to the remainder of the molecule and R is hydrogen, hydrocarbyl, or substituted hydrocarbyl.
  • acrylic denotes a moiety having the structural formula H 2 C ⁇ CH—C(O)O—*, where * denotes the point of attachment of the moiety to the remainder of the molecule.
  • the term “adult” refers to an individual over 18 years of age.
  • alicyclic means a saturated monocyclic group of 3 to 8 carbon atoms and includes cyclopentyl, cyclohexyl, cycloheptyl, and the like.
  • aliphatic denotes saturated and non-aromatic unsaturated hydrocarbyl moieties having, for example, one to about twenty carbon atoms or, in specific embodiments, one to about twelve carbon atoms, one to about ten carbon atoms, one to about eight carbon atoms, or even one to about four carbon atoms.
  • the aliphatic groups include, for example, alkyl moieties such as methyl, ethyl, n-propyl, isopropyl, n-butyl, isobutyl, sec-butyl, tert-butyl, pentyl, iso-amyl, hexyl and the like, and alkenyl moieties of comparable chain length.
  • alkanol denotes an alkyl moiety that has been substituted with at least one hydroxyl group.
  • alkanol groups are “lower alkanol” groups comprising one to six carbon atoms, one of which is attached to an oxygen atom.
  • lower alkanol groups comprise one to three carbon atoms.
  • alkenyl group encompasses linear or branched carbon radicals having at least one carbon-carbon double bond.
  • alkenyl group can encompass conjugated and non-conjugated carbon-carbon double bonds or combinations thereof.
  • An alkenyl group for example and without being limited thereto, can encompass two to about twenty carbon atoms or, in a particular embodiment, two to about twelve carbon atoms.
  • alkenyl groups are “lower alkenyl” groups having two to about four carbon atoms. Examples of alkenyl groups include, but are not limited thereto, ethenyl, propenyl, allyl, vinyl, butenyl and 4-methylbutenyl.
  • alkenyl group and “lower alkenyl group” encompass groups having “cis” or “trans” orientations, or alternatively, “E” or “Z” orientations.
  • alkyl group as used, either alone or within other terms such as “haloalkyl group,” “aminoalkyl group” and “alkylamino group”, encompasses saturated linear or branched carbon radicals having, for example, one to about twenty carbon atoms or, in specific embodiments, one to about twelve carbon atoms. In other embodiments, alkyl groups are “lower alkyl” groups having one to about six carbon atoms.
  • lower alkyl groups have one to four carbon atoms.
  • alkylamino group refers to amino groups directly attached to the remainder of the molecule via the nitrogen atom of the amino group and wherein the nitrogen atom of the alkylamino group is substituted by one or two alkyl groups.
  • alkylamino groups are “lower alkylamino” groups having one or two alkyl groups of one to six carbon atoms, attached to a nitrogen atom. In other embodiments, lower alkylamino groups have one to three carbon atoms.
  • Suitable “alkylamino” groups may be mono or dialkylamino such as N-methylamino, N-ethylamino, N,N-dimethylamino, N,N-diethylamino, pentamethyleneamine and the like.
  • allyl denotes a moiety having the structural formula H 2 C ⁇ CH—CH 2 —, where * denotes the point of attachment of the moiety to the remainder of the molecule and the point of attachment is to a heteroatom or an aromatic moiety.
  • allylamine denotes a moiety having the structural formula H 2 C ⁇ CH—CH 2 N(X 8 )(X 9 ), wherein X 8 and X 9 are independently hydrogen, hydrocarbyl, or substituted hydrocarbyl, or X 8 and X 9 taken together form a substituted or unsubstituted alicyclic, aryl, or heterocyclic moiety, each as defined in connection with such term, typically having from 3 to 8 atoms in the ring.
  • amine or “amino” as used alone or as part of another group, represents a group of formula —N(X 8 )(X 9 ), wherein X 8 and X 9 are independently hydrogen, hydrocarbyl, or substituted hydrocarbyl, heteroaryl, or heterocyclo, or X 8 and X 9 taken together form a substituted or unsubstituted alicyclic, aryl, or heterocyclic moiety, each as defined in connection with such term, typically having from 3 to 8 atoms in the ring.
  • aminoalkyl group encompasses linear or branched alkyl groups having one to about ten carbon atoms, any one of which may be substituted with one or more amino groups, directly attached to the remainder of the molecule via an atom other than a nitrogen atom of the amine group(s).
  • the aminoalkyl groups are “lower aminoalkyl” groups having one to six carbon atoms and one or more amino groups. Examples of such groups include aminomethyl, aminoethyl, aminopropyl, aminobutyl and aminohexyl.
  • anion exchange material and “cation exchange material” take their normal meaning in the art.
  • anion exchange material and “cation exchange material” refer to materials that exchange anions and cations, respectively.
  • Anion and cation exchange materials are typically water-insoluble substances which can exchange some of their cations or anions, respectively, for similarly charged anions or cations contained in a medium with which they are in contact.
  • Anion exchange materials may contain positively charged groups, which are fixed to the backbone materials and allow passage of anions but reject cations. A non-exhaustive list of such positively charged groups includes: amino group, alkyl substituted phosphine, and alkyl substituted sulphides.
  • a non-exhaustive list of cation or anion exchange materials includes: clays (e.g., bentonite, kaolinite, and illite), vermiculite, zeolites (e.g., analcite, chabazite, sodalite, and clinoptilolite), synthetic zeolites, polybasic acid salts, hydrous oxides, metal ferrocyanides, and heteropolyacids.
  • Cation exchange materials can contain negatively charged groups fixed to the backbone material, which allow the passage of cations but reject anions.
  • a non-exhaustive list of such negatively charged groups includes: sulphate, carboxylate, phosphate, and benzoate.
  • aromatic group or “aryl group” means an aromatic group having one or more rings wherein such rings may be attached together in a pendent manner or may be fused.
  • an aromatic group is one, two or three rings.
  • Monocyclic aromatic groups may contain 5 to 10 carbon atoms, typically 5 to 7 carbon atoms, and more typically 5 to 6 carbon atoms in the ring.
  • Typical polycyclic aromatic groups have two or three rings.
  • Polycyclic aromatic groups having two rings typically have 8 to 12 carbon atoms, preferably 8 to 10 carbon atoms in the rings.
  • aromatic groups include, but are not limited to, phenyl, naphthyl, tetrahydronaphthyl, indanyl, biphenyl, phenanthryl, anthryl or acenaphthyl.
  • bead is used to describe a crosslinked polymer that is substantially spherical in shape.
  • bicarbonate equivalent is used to describe an organic acid or anion that yields bicarbonate when metabolized. Citrate and succinate are exemplary bicarbonate equivalents.
  • binding as used herein in connection with a polymer and one or more ions, that is, a cation (e.g. “proton-binding” polymer) and an anion, is an “ion-binding” polymer and/or when it associates with the ion, generally though not necessarily in a non-covalent manner, with sufficient association strength that at least a portion of the ion remains bound under the in vitro or in vivo conditions in which the polymer is used for sufficient time to effect a removal of the ion from solution or from the body.
  • ceramic material takes its normal meaning in the art.
  • the term “ceramic material” refers to an inorganic, nonmetallic, solid material comprising metal, nonmetal or metalloid atoms primarily held in ionic and covalent bonds.
  • a non-exhaustive list of examples of ceramic materials includes: barium titanate, bismuth strontium calcium copper oxide, boron oxide, earthenware, ferrite, lanthanum carbonate, lead zirconate, titanate, magnesium diboride, porcelain, sialon, silicon carbide, silicon nitride, titanium carbide, yttrium barium copper oxide, zinc oxide, zirconium dioxide, and partially stabilised zirconia.
  • the term “clinically significant increase” as used herein in connection with a treatment refers to a treatment that improves or provides a worthwhile change in an individual from a dysfunctional state back to a relatively normal functioning state, or moves the measurement of that state in the direction of normal functioning, or at least a marked improvement to untreated.
  • a number of methods can be used to calculate clinical significance.
  • a non-exhaustive list of methods for calculating clinical significance includes: Jacobson-Truax, Gulliksen-Lord-Novick, Edwards-Nunnally, Hageman-Arrindell, and Hierarchical Linear Modeling (HLM).
  • crosslink density denotes the average number of connections of the amine containing repeat unit to the rest of the polymer.
  • the number of connections can be 2, 3, 4 and higher. Repeat units in linear, non-crosslinked polymers are incorporated via 2 connections. To form an insoluble gel, the number of connections should be greater than 2.
  • Low crosslinking density materials such as sevelamer have on average about 2.1 connections between repeat units. More crosslinked systems such as bixalomer have on average about 4.6 connections between the amine-containing repeat units.
  • Crosslinking density represents a semi-quantitative measure based on the ratios of the starting materials used. Limitations include the fact that it does not account for different crosslinking and polymerization methods.
  • small molecule amine systems require higher amounts of crosslinker as the crosslinker also serves as the monomer to form the polymer backbone whereas for radical polymerizations the polymer chain is formed independent from the crosslinking reaction. This can lead to inherently higher crosslinking densities under this definition for the substitution polymerization/small molecule amines as compared to radical polymerization crosslinked materials.
  • crosslinker encompasses hydrocarbyl or substituted hydrocarbyl, linear or branched molecules capable of reacting with any of the described monomers, or the infinite polymer network, as described in Formula 1, more than one time.
  • the reactive group in the crosslinker can include, but is not limited to alkyl halide, epoxide, phosgene, anhydride, carbamate, carbonate, isocyanate, thioisocyanate, esters, activated esters, carboxylic acids and derivatives, sulfonates and derivatives, acyl halides, aziridines, ⁇ , ⁇ -unsaturated carbonyls, ketones, aldehydes, pentafluoroaryl groups, vinyl, allyl, acrylate, methacrylate, acrylamide, methacrylamide, styrenic, acrylonitriles and combinations thereof.
  • the crosslinker's reactive group will include alkyl halide, epoxide, anhydrides, isocyanates, allyl, vinyl, acrylamide, and combinations thereof. In one such embodiment, the crosslinker's reactive group will be alkyl halide, epoxide, or allyl.
  • diallylamine denotes an amino moiety having two allyl groups.
  • dry bead and “dry polymer” refer to beads or polymers that contain no more than 5% by weight of a non-polymer swelling agent or solvent. Often the swelling agent/solvent is water remaining at the end of a purification. This is generally removed by lyophilization or oven drying before storage or further crosslinking of a preformed amine polymer. The amount of swelling agent/solvent can be measured by heating (e.g., heating to 100-200° C.) and measuring the resulting change in weight. This is referred to a “loss on drying” or “LOD.”
  • eGFR estimated glomerular filtration rate
  • Creatinine is a commonly used endogenous filtration marker in clinical practice and several equations have been proposed for estimating the glomerular filtration rate.
  • all eGFR values may be determined according to the CKD-EPI equation (Levey et al., A New Equation to Estimate Glomerular Filtration Rate. Ann Intern Med. 2009; 150:604-612):
  • GFR 41*min(Scr/ ⁇ ,1) ⁇ *max(Scr/ ⁇ ,1) ⁇ 1.209 *0.993 Age *1.018 [if female]*1.159 [if black]
  • Scr is serum creatinine (mg/dL)
  • is 0.7 for females and 0.9 for males
  • is ⁇ 0.329 for females and ⁇ 0.411 for males
  • min indicates the minimum of Scr/ ⁇ or 1
  • max indicates the maximum of Scr/ ⁇ or 1.
  • ethereal denotes a moiety having an oxygen bound to two separate carbon atoms as depicted the structural formula *—H x C—O—CH x —*, where * denotes the point of attachment to the remainder of the moiety and x independently equals 0, 1, 2, or 3.
  • gel is used to describe a crosslinked polymer that has an irregular shape.
  • GFR glomerular filtration rate
  • halo means halogens such as fluorine, chlorine, bromine or iodine atoms.
  • haloalkyl group encompasses groups wherein any one or more of the alkyl carbon atoms is substituted with halo as defined above. Specifically encompassed are monohaloalkyl, dihaloalkyl and polyhaloalkyl groups including perhaloalkyl.
  • a monohaloalkyl group for example, may have either an iodo, bromo, chloro or fluoro atom within the group.
  • Dihalo and polyhaloalkyl groups may have two or more of the same halo atoms or a combination of different halo groups.
  • “Lower haloalkyl group” encompasses groups having 1-6 carbon atoms.
  • lower haloalkyl groups have one to three carbon atoms.
  • haloalkyl groups include fluoromethyl, difluoromethyl, trifluoromethyl, chloromethyl, dichloromethyl, trichloromethyl, pentafluoroethyl, heptafluoropropyl, difluorochloromethyl, dichlorofluoromethyl, difluoroethyl, difluoropropyl, dichloroethyl and dichloropropyl.
  • heteroaliphatic describes a chain of 1 to 25 carbon atoms, typically 1 to 12 carbon atoms, more typically 1 to 10 carbon atoms, and most typically 1 to 8 carbon atoms, and in some embodiments 1 to 4 carbon atoms that can be saturated or unsaturated (but not aromatic), containing one or more heteroatoms, such as halogen, oxygen, nitrogen, sulfur, phosphorus, or boron.
  • a heteroatom atom may be a part of a pendant (or side) group attached to a chain of atoms (e.g., —CH(OH)—CH(NH 2 )— where the carbon atom is a member of a chain of atoms) or it may be one of the chain atoms (e.g., —ROR— or —RNHR— where each R is aliphatic).
  • Heteroaliphatic encompasses heteroalkyl and heterocyclo but does not encompass heteroaryl.
  • heteroalkyl describes a fully saturated heteroaliphatic moiety.
  • heteroaryl means a monocyclic or bicyclic aromatic radical of 5 to 10 ring atoms, unless otherwise stated, where one or more, (in one embodiment, one, two, or three), ring atoms are heteroatom selected from N, O, or S, the remaining ring atoms being carbon.
  • Representative examples include, but are not limited to, pyrrolyl, thienyl, thiazolyl, imidazolyl, furanyl, indolyl, isoindolyl, oxazolyl, isoxazolyl, benzothiazolyl, benzoxazolyl, quinolinyl, isoquinolinyl, pyridinyl, pyrimidinyl, pyrazinyl, pyridazinyl, triazolyl, tetrazolyl, and the like.
  • heteroaryl and “aryl” are mutually exclusive.
  • Heteroarylene means a divalent heteroaryl radical.
  • heteroatom means an atom other than carbon and hydrogen. Typically, but not exclusively, heteroatoms are selected from the group consisting of halogen, sulfur, phosphorous, nitrogen, boron and oxygen atoms. Groups containing more than one heteroatom may contain different heteroatoms.
  • heterocyclo means a saturated or unsaturated group of 4 to 8 ring atoms in which one or two ring atoms are heteroatom such as N, O, B, P and S(O) n , where n is an integer from 0 to 2, the remaining ring atoms being carbon. Additionally, one or two ring carbon atoms in the heterocyclyl ring can optionally be replaced by a —C(O)— group.
  • heterocyclyl includes, but is not limited to, pyrrolidino, piperidino, homopiperidino, 2-oxopyrrolidinyl, 2-oxopiperidinyl, morpholino, piperazino, tetrahydro-pyranyl, thiomorpholino, and the like.
  • heterocyclyl ring is unsaturated it can contain one or two ring double bonds provided that the ring is not aromatic.
  • heterocyclyl group contains at least one nitrogen atom, it is also referred to herein as heterocycloamino and is a subset of the heterocyclyl group.
  • hydrocarbon group or “hydrocarbyl group” means a chain of 1 to 25 carbon atoms, typically 1 to 12 carbon atoms, more typically 1 to 10 carbon atoms, and most typically 1 to 8 carbon atoms. Hydrocarbon groups may have a linear or branched chain structure. Typical hydrocarbon groups have one or two branches, typically one branch. Typically, hydrocarbon groups are saturated. Unsaturated hydrocarbon groups may have one or more double bonds, one or more triple bonds, or combinations thereof. Typical unsaturated hydrocarbon groups have one or two double bonds or one triple bond; more typically unsaturated hydrocarbon groups have one double bond.
  • Initiator is a term used to describe a reagent that initiates a polymerization.
  • measured glomerular filtration rate refers to a measurement of the glomerular filtration rate using any chemical (e.g., inulin, iothalamate, iohexol, etc.) that has a steady level in the blood, and is freely filtered but neither reabsorbed nor secreted by the kidneys according to standard technique.
  • chemical e.g., inulin, iothalamate, iohexol, etc.
  • Michael acceptor takes its normal meaning in the art.
  • the term “Michael acceptor” refers to activated olefins, such as ⁇ , ⁇ -unsaturated carbonyl compounds.
  • a Michael acceptor can be a conjugated system with an electron withdrawing group, such as cyano, keto or ester.
  • An electron withdrawing group such as cyano, keto or ester.
  • a non-exhaustive list of examples of Michael acceptors includes: vinyl ketones, alkyl acrylates, acrylo nitrile, and fumarates.
  • MW/N molecular weight per nitrogen
  • nonabsorbable takes its normal meaning in the art. Therefore, if something is nonabsorbable it is not absorbed during its passage through the human GI tract. This could be measured by any appropriate means.
  • One option known to the skilled person would be to examine faeces to see if the nonabsorbable material is recovered after passing through the GI tract. As a practical matter, the amount of a nonabsorbable material recovered in this scenario will never be 100% of the material administered. For example, about 90-99% of the material might be recovered from the faeces.
  • Nonabsorbable compositions may be particulate compositions that are essentially insoluble in the human GI tract and have a particle size that is large enough to avoid passive or active absorption through the human GI tract.
  • nonabsorbable compositions is meant to imply that the substance does not enter the lymph, blood, interstitial fluids or organs through the main entry points of the human GI tract, namely by paracellular entry between gut epithelial cells, by endocytic uptake through gut epithelial cells, or through entry via M cells comprising the gut epithelial antigen sampling and immune surveillance system (Jung, 2000), either through active or passive transport processes.
  • heterocyclyl group optionally substituted with an alkyl group means that the alkyl may but need not be present, and the description includes embodiments in which the heterocyclyl group is substituted with an alkyl group and embodiments in which the heterocyclyl group is not substituted with alkyl.
  • Particle size is measured by wet laser diffraction using Mie theory. Particles are dispersed in an appropriate solvent, such as water or methanol, and added to the sample chamber to achieve red channel obscuration of 10-20%. Sonication may be performed, and a dispersing agent, such as a surfactant (e.g. Tween-80), may be added in order to disrupt weak particle-particle interactions.
  • a dispersing agent such as a surfactant (e.g. Tween-80)
  • the refractive index setting of the particles used for size distribution calculation is selected to minimize artifacts in the results and the R parameter value, determined by the laser diffraction software.
  • the D(0.1), D(0.5), and D(0.9) values characterizing the particle size distribution by volume-basis are recorded.
  • “Pharmaceutically acceptable” as used in connection with a carrier, diluent or excipient means a carrier, diluent or an excipient, respectively, that is useful in preparing a pharmaceutical composition that is generally safe, non-toxic and neither biologically nor otherwise undesirable for veterinary use and/or human pharmaceutical use.
  • post polymerization crosslinking is a term that describes a reaction to an already formed bead or gel, where more crosslinking is introduced to the already formed bead or gel to create a bead or gel that has an increased amount of crosslinking.
  • post polymerization modification is a term that describes a modification to an already formed bead or gel, where a reaction or a treatment introduces an additional functionality. This functionality can be linked either covalently or non-covalently to the already formed bead.
  • QAA quaternized amine assay
  • the free-amine polymer being tested is prepared at a concentration of 2.5 mg/ml (e.g. 25 mg dry mas) in 10 mL of QAA buffer.
  • the mixture is incubated at 37° C. for ⁇ 16 hours with agitation on a rotisserie mixer. After incubation and mixing, 600 microliters of supernatant is removed and filtered using a 800 microliter, 0.45 micrometer pore size, 96-well poly propylene filter plate. With the samples arrayed in the filter plate and the collection plate fitted on the bottom, the unit is centrifuged at 1000 ⁇ g for 1 minute to filter the samples. After filtration into the collection plate, the respective filtrates are diluted appropriately before measuring for chloride content.
  • the IC method e.g. ICS-2100 Ion Chromatography, Thermo Fisher Scientific
  • Thermo Fisher Scientific used for the analysis of chloride content in the filtrates consists of a 15 mM KOH mobile phase, an injection volume of 5 microliters, with a run time of three minutes, a washing/rinse volume of 1000 microliters, and flow rate of 1.25 mL/min.
  • Binding ⁇ ⁇ capacity ⁇ ⁇ expressed ⁇ ⁇ as ⁇ ⁇ mmol ⁇ ⁇ chloride ⁇ / ⁇ g ⁇ ⁇ dry ⁇ ⁇ polymer ( Cl ⁇ ⁇ start - Cl ⁇ ⁇ eq ) 2.5
  • Cl start corresponds to the starting concentration of chloride in the QAA buffer
  • Cl eq corresponds to the equilibrium value of chloride in the measured filtrates after exposure to the test polymer
  • 2.5 is the polymer concentration in mg/ml.
  • short chain carboxylic acid or “short chain fatty acid” take their normal meaning in the art.
  • the terms “short chain carboxylic acid” or “short chain fatty acid” refer to carboxylic acids having a chain length of 0, 1, 2, 3, 4, 5 or 6 carbon atoms long.
  • a non-exhaustive list of examples of short chain carboxylic acids includes: formic acid, acetic acid, propionic acid, butyric acid, isobutyric acid, valeric acid, isovaleric acid, and lactic acid.
  • Simulated Gastric Fluid or “SGF” Assay describes a test to determine total chloride binding capacity for a test polymer using a defined buffer that simulates the contents of gastric fluid as follows: Simulated gastric fluid (SGF) consists of 35 mM NaCl, 63 mM HCl, pH 1.2. To perform the assay, the free-amine polymer being tested is prepared at a concentration of 2.5 mg/ml (25 mg dry mass) in 10 mL of SGF buffer. The mixture is incubated at 37° C. overnight for ⁇ 12-16 hours with agitation on a rotisserie mixer. Unless another time period is otherwise stated, SGF binding data or binding capacities recited herein are determined in a time period of this duration.
  • the tubes containing the polymer are centrifuged for 2 minutes at 500-1000 ⁇ g to pellet the test samples. Approximately 750 microliters of supernatant are removed and filtered using an appropriate filter, for example a 0.45 micrometer pore-size syringe filter or an 800 microliter, 1 micrometer pore-size, 96-well, glass filter plate that has been fitted over a 96-well 2 mL collection plate.
  • an appropriate filter for example a 0.45 micrometer pore-size syringe filter or an 800 microliter, 1 micrometer pore-size, 96-well, glass filter plate that has been fitted over a 96-well 2 mL collection plate.
  • the unit With the samples arrayed in the filter plate and the collection plate fitted on the bottom, the unit is centrifuged at 1000 ⁇ g for 1 minute to filter the samples.
  • a syringe filter may be used in lieu of the filter plate, to retrieve ⁇ 2-4 mL of filtrate into a 15 mL container.
  • the respective filtrates are diluted 4 ⁇ with water and the chloride content of the filtrate is measured via ion chromatography (IC).
  • IC ion chromatography
  • Dionex ICS-2100 Thermo Scientific
  • ICS-2100 Thermo Scientific
  • Binding capacity expressed as mmol chloride/g polymer where CI start corresponds to the starting concentration of chloride in the SGF buffer, Cl eq corresponds to the equilibrium value of chloride in the diluted measured filtrates after exposure to the test polymer, 4 is the dilution factor and 2.5 is the polymer concentration in mg/ml.
  • SIB “Simulated Small Intestine Inorganic Buffer” or “SIB” is a test to determine the chloride and phosphate binding capacity of free amine test polymers in a selective specific interfering buffer assay (SIB).
  • the buffer used for the SIB assay comprises 36 mM NaCl, 20 mM NaH 2 PO 4 , 50 mM 2-(N-morpholino)ethanesulfonic acid (MES) buffered to pH 5.5.
  • MES 2-(N-morpholino)ethanesulfonic acid
  • the SIB buffer contains concentrations of chloride, phosphate and pH that are present in the human duodenum and upper gastrointestinal tract (Stevens T, Conwell D L, Zuccaro G, Van Lente F, Khandwala F, Purich E, et al. Electrolyte composition of endoscopically collected duodenal drainage fluid after synthetic porcine secretin stimulation in healthy subjects. Gastrointestinal endoscopy. 2004; 60(3):351-5, Fordtran J, Locklear T. Ionic constituents and osmolality of gastric and small-intestinal fluids after eating. Digest Dis Sci. 1966; 11(7):503-21) and is an effective measure of the selectivity of chloride binding compared to phosphate binding by a polymer.
  • the free amine polymer being tested is prepared at a concentration of 2.5 mg/ml (25 mg dry mass) in mL of SIB buffer.
  • the mixture is incubated at 37° C. for 1 hour with agitation on a rotisserie mixer. Unless another time period is otherwise stated, SIB binding data or binding capacities recited herein are determined in a time period of this duration.
  • the tubes containing the polymer are centrifuged for 2 minutes at 1000 ⁇ g to pellet the test samples.
  • a syringe filter (0.45 micrometer) may be used in lieu of the filter plate, to retrieve ⁇ 2-4 mL of filtrate into a 15 mL vial.
  • the respective filtrates are diluted before measuring for chloride or phosphate content.
  • the filtrates under analysis are diluted 4 ⁇ with water.
  • the chloride and phosphate content of the filtrate is measured via ion chromatography (IC).
  • IC ion chromatography
  • Dionex ICS-2100 Thermo Scientific
  • ICS-2100 Thermo Scientific
  • Binding ⁇ ⁇ capacity ⁇ ⁇ expressed ⁇ ⁇ as ⁇ ⁇ mmol ⁇ ⁇ chloride ⁇ / ⁇ g ⁇ ⁇ polymer ( Cl start - Cl final ) ⁇ 4 2.5
  • Cl start corresponds to the starting concentration of chloride in the SIB buffer
  • Cl final corresponds to the final value of chloride in the measured diluted filtrates after exposure to the test polymer
  • 4 is the dilution factor
  • 2.5 is the polymer concentration in mg/ml.
  • Binding ⁇ ⁇ capacity ⁇ ⁇ expressed ⁇ ⁇ as ⁇ ⁇ mmol ⁇ ⁇ p ⁇ hosphate ⁇ / ⁇ g ⁇ ⁇ polymer ( P start - P final ) ⁇ 4 2.5
  • P start corresponds to the starting concentration of phosphate in the SIB buffer
  • P final corresponds to the final value of phosphate in the measured diluted filtrates after exposure to the test polymer
  • 4 is the dilution factor
  • 2.5 is the polymer concentration in mg/ml.
  • the term “statistically significant” refers to the likelikhood that a relationship between two or more variables is caused by something other than random chance. More precisely, the significance level, ⁇ , defined for a study is the probability of the study rejecting the null hypothesis, given that it were true, and the p-value, p, of a result is the probability of obtaining a result at least as extreme, given that the null hypothesis were true. The result is statistically significant, by the standards of the study, when p ⁇ . The significance level for a study is chosen before data collection, and typically set to 5%
  • substituted hydrocarbyl denotes hydrocarbyl, alkyl, alkenyl, aryl, heterocyclo, or heteroaryl moieties which are substituted with at least one atom other than carbon and hydrogen, including moieties in which a carbon chain atom is substituted with a hetero atom such as nitrogen, oxygen, silicon, phosphorous, boron, sulfur, or a halogen atom.
  • substituents include halogen, heterocyclo, alkoxy, alkenoxy, alkynoxy, aryloxy, hydroxy, keto, acyl, acyloxy, nitro, amino, amido, nitro, cyano, thiol, ketals, acetals, esters and ethers.
  • “Swelling Ratio” or simply “Swelling” describes the amount of water absorbed by a given amount of polymer divided by the weight of the polymer aliquot.
  • the method used to determine the Swelling Ratio for any given polymer comprised the following:
  • a “target ion” is an ion to which the polymer binds, and usually refers to the major ions bound by the polymer, or the ions whose binding to the polymer is thought to produce the therapeutic effect of the polymer (e.g., proton and chloride binding which leads to net removal of HCl).
  • theoretical capacity represents the calculated, expected binding of hydrochloric acid in an “SGF” assay, expressed in mmol/g.
  • the theoretical capacity is based on the assumption that 100% of the amines from the monomer(s) and crosslinker(s) are incorporated in the crosslinked polymer based on their respective feed ratios. Theoretical capacity is thus equal to the concentration of amine functionalities in the polymer (mmol/g).
  • the theoretical capacity assumes that each amine is available to bind the respective anions and cations and is not adjusted for the type of amine formed (e.g. it does not subtract capacity of quaternary amines that are not available to bind proton).
  • “Therapeutically effective amount” means the amount of a proton-binding crosslinked polymer that, when administered to a patient for treating a disease, is sufficient to effect such treatment for the disease.
  • the amount constituting a “therapeutically effective amount” will vary depending on the polymer, the severity of the disease and the age, weight, etc., of the mammal to be treated.
  • Treating” or “treatment” of a disease includes (i) inhibiting the disease, i.e., arresting or reducing the development of the disease or its clinical symptoms; or (ii) relieving the disease, i.e., causing regression of the disease or its clinical symptoms. Inhibiting the disease, for example, would include prophylaxis.
  • triallylamine denotes an amino moiety having three allyl groups.
  • weight percent crosslinker represents the calculated percentage, by mass, of a polymer sample that is derived from the crosslinker. Weight percent crosslinker is calculated using the feed ratio of the polymerization, and assumes full conversion of the monomer and crosslinker(s). The mass attributed to the crosslinker is equal to the expected increase of molecular weight in the infinite polymer network after reaction (e.g., 1,3-dichloropropane is 113 amu, but only 42 amu are added to a polymer network after crosslinking with DCP because the chlorine atoms, as leaving groups, are not incorporated into the polymer network).
  • acid-base disorders may be treated using pharmaceutical compositions comprising a nonabsorbable composition having the capacity to remove clinically significant quantities of protons, the conjugate base of one or more strong acids, and/or one or more strong acids.
  • An individual afflicted with a an acute or chronic acid/base disorder characterized by a baseline serum bicarbonate value of less than 22 mEq/l may thus be treated by oral administration of a pharmaceutical composition comprising the nonabsorbable composition which then transits the individual's digestive system, binds a target species (protons, one or more conjugate base(s) of a strong acid and/or one or more strong acid(s)) as it transits the digestive system, and removes the bound target species by normal biological function (defecation).
  • the individual afflicted with an acute or chronic acid/base disorder may be at any stage of chronic kidney disease.
  • the afflicted individual has not yet reached end stage renal disease (“ESRD”) sometimes also referred to as end stage chronic kidney disease and is not yet on dialysis (i.e., the individual has a mGFR (or eGFR) of at least 15 mL/min/1.73 m 2 ).
  • the afflicted individual will be Stage 3B CKD (i.e., the individual has a mGFR (or eGFR) in the range of 30-44 mL/min/1.73 m 2 for at least three months).
  • the afflicted individual will be Stage 3A CKD (i.e., the individual has a mGFR (or eGFR) in the range of 45-59 mL/min/1.73 m 2 for at least three months).
  • the afflicted individual has a mGFR or an eGFR of less than 60 ml/min/1.73 m 2 for at least three months.
  • the afflicted individual has a mGFR or an eGFR of less than 45 mL/min/1.73 m 2 for at least three months.
  • the afflicted individual has a mGFR or an eGFR of less than 30 mL/min/1.73 m 2 for at least three months.
  • the the afflicted individual has a mGFR or an eGFR of 15-30, 15-45, 15-60, 30-45 or even 30-60 mL/min/1.73 m 2 for at least three months.
  • the baseline serum bicarbonate value may be the serum bicarbonate concentration determined at a single time point or may be the mean or median value of two or more serum bicarbonate concentrations determined at two or more time-points.
  • the baseline serum bicarbonate value may be the value of the serum bicarbonate concentration determined at a single time point and the baseline serum bicarbonate value is used as a basis to determine an acute acidic condition requiring immediate treatment.
  • the baseline serum bicarbonate treatment value is the mean value of the serum bicarbonate concentration for serum samples drawn at different time points (e.g., different days).
  • the baseline serum bicarbonate treatment value is the mean value of the serum bicarbonate concentration for serum samples drawn on different days (e.g., at least 2, 3, 4, 5 or more days, that may be consecutive or separated by one or more days or even weeks).
  • the baseline serum bicarbonate treatment value is the mean value of the serum bicarbonate concentration for serum samples drawn on two consecutive days preceding the initiation of treatment.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 21 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 20 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 19 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 18 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 17 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 16 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 15 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 14 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 13 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 12 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 11 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 10 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of less than 9 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value of at least 9 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 10 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 11 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 12 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 13 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 14 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 15 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 16 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 17 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 18 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 19 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 20 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value of at least 21 mEq/l.
  • the acid-base disorder being treated is characterized by a baseline serum bicarbonate value in the range of 9 to 21 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 12 to 20 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 12 to 19 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 12 to 18 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 12 to 17 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 12 to 16 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 9 to 11 mEq/l.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 12-14.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 15-17.
  • the acid-base disorder is characterized by a baseline serum bicarbonate value in the range of 18-21.
  • oral administration of a pharmaceutical composition containing a nonabsorbable composition increases the individual's serum bicarbonate value from baseline to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 1 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 1.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 2 mEq/l.
  • the treatment the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 2.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least at least 3 mEq/l.
  • the treatment increases the baseline serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 3.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 4 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 5 mEq/l but does not exceed 29 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 5 mEq/l but does not exceed 28 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 5 mEq/l but does not exceed 27 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 5 mEq/l but does not exceed 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 6 mEq/l but does not exceed 29 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 6 mEq/l but does not exceed 28 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 6 mEq/l but does not exceed 27 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 6 mEq/l but does not exceed 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 7 mEq/l but does not exceed 29 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 7 mEq/l but does not exceed 28 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 7 mEq/l but does not exceed 27 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 7 mEq/l but does not exceed 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 8 mEq/l but does not exceed 29 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 8 mEq/l but does not exceed 28 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 8 mEq/l but does not exceed 27 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 8 mEq/l but does not exceed 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 9 mEq/l but does not exceed 29 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 9 mEq/l but does not exceed 28 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 9 mEq/l but does not exceed 27 mEq/l.
  • the treatment increases the individual's serum bicarbonate value to an increased serum bicarbonate value that exceeds the baseline serum bicarbonate value by at least 9 mEq/l but does not exceed 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • treatment with the nonabsorbable composition increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 1 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 1.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 2 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 2.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 3 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 3.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 4 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 4.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 5.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 20 mEq/l by at least 6 mEq/l.
  • the increased serum bicarbonate value preferably does not exceed 29 mEq/l.
  • the increased serum bicarbonate value may not exceed 28 mEq/l.
  • the increased serum bicarbonate value may not exceed 27 mEq/l.
  • the increased serum bicarbonate value may not exceed 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • treatment with the nonabsorbable composition increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 1 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 1.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 2 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 2.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 3 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 3.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 4 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 4.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 5.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 9 to 21 mEq/l by at least 6 mEq/l.
  • the increased serum bicarbonate value preferably does not exceed 29 mEq/l.
  • the increased serum bicarbonate value may not exceed 28 mEq/l.
  • the increased serum bicarbonate value may not exceed 27 mEq/l.
  • the increased serum bicarbonate value may not exceed 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • the acid-base disorder is treated with a pharmaceutical composition comprising the nonabsorbable composition and the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 1 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 1.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 2 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 2.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 3 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 3.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 4 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 4.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 6 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 7 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 8 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l by at least 9 mEq/l.
  • the increased serum bicarbonate value preferably does not exceed 29 mEq/l.
  • the increased serum bicarbonate value may not exceed 28 mEq/l.
  • the increased serum bicarbonate value may not exceed 27 mEq/l.
  • the increased serum bicarbonate value may not exceed 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 1 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 1.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 2 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 2.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 3 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 3.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 4 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 4.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 6 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 7 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 8 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l by at least 9 mEq/l.
  • the increased serum bicarbonate value preferably does not exceed 29 mEq/l.
  • the increased serum bicarbonate value may not exceed 28 mEq/l.
  • the increased serum bicarbonate value may not exceed 27 mEq/l.
  • the increased serum bicarbonate value may not exceed 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 1 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 1.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 2 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 2.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 3 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 3.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 4 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 4.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 5.5 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l by at least 6 mEq/l.
  • the increased serum bicarbonate value preferably does not exceed 29 mEq/l.
  • the increased serum bicarbonate value may not exceed 28 mEq/l.
  • the increased serum bicarbonate value may not exceed 27 mEq/l.
  • the increased serum bicarbonate value may not exceed 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 21 mEq/l to an increased value in the range of 22 mEq/l to 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 17 mEq/l to an increased value in the range of 22 mEq/l to 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 12 to 14 mEq/l to an increased value in the range of 22 mEq/l to 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 15 to 17 mEq/l to an increased value in the range of 22 mEq/l to 26 mEq/l.
  • the treatment increases the individual's serum bicarbonate value from a baseline serum bicarbonate value in the range of 18 to 21 mEq/l to an increased value in the range of 22 mEq/l to 26 mEq/l.
  • the treatment enables the increased serum bicarbonate value to be sustained over a prolonged period of at least one week, at least one month, at least two months, at least three months, at least six months, or even at least one year.
  • the treatment achieves a clinically significant increase is achieved within a treatment period of less than one month.
  • the treatment achieves a clinically significant increase within a treatment period of 25 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 3 weeks.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 15 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 2 weeks.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 10 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 1 week.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 6 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 5 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 4 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 3 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 2 days.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 1 day.
  • the treatment achieves the clinically significant increase is achieved within a treatment period of 12 hours.
  • the treatment achieves a clinically significant increase is achieved without any change in the individual's diet or dietary habits relative to the period immediately preceding the initiation of treatment.
  • the clinically significant increase is achieved independent of the individual's diet or dietary habits.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2.5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 2 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1.5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value returns to the baseline value ⁇ 1 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 1 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 1 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 1 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 1.5 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 2 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 2 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 2 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 2.5 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 3 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 3 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 3 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 3.5 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 4 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 4 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 4 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 4.5 mEq/l within 12 hours of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 1 month of the cessation of treatment. For example, in one such embodiment. For example, in one such embodiment the individual's serum bicarbonate value decreases by at least 5 mEq/l within 3 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 5 mEq/l within 2 weeks of the cessation of treatment. By way of further example, in one such embodiment the individual's serum bicarbonate value decreases by at least 5 mEq/l within 10 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 9 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 8 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 7 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 6 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 5 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 4 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 3 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 2 days of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 1 day of the cessation of treatment.
  • the individual's serum bicarbonate value decreases by at least 5 mEq/l within 12 hours of the cessation of treatment.
  • the baseline serum bicarbonate value is the value of the serum bicarbonate concentration determined at a single time point. In another embodiment, the baseline serum bicarbonate value is the mean value of at least two serum bicarbonate concentrations determined at different time-points. For example, in one such embodiment the baseline serum bicarbonate value is the mean value of at least two serum bicarbonate concentrations for serum samples drawn on different days. By way of further example, the baseline serum bicarbonate value is the mean or median value of at least two serum bicarbonate concentrations for serum samples drawn on non-consecutive days. By way of further example, in one such method the non-consecutive days are separated by at least two days. By way of further example, in one such method the non-consecutive days are separated by at least one week. By way of further example, in one such method the non-consecutive days are separated by at least two weeks. By way of further example, in one such method the non-consecutive days are separated by at least three weeks.
  • the daily dose is no more than 100 g/day of the nonabsorbable composition.
  • the daily dose is no more than 90 g/day of the nonabsorbable composition.
  • the daily dose is no more than 75 g/day of the nonabsorbable composition.
  • the daily dose is no more than 65 g/day of the nonabsorbable composition.
  • the daily dose is no more than 50 g/day of the nonabsorbable composition.
  • the daily dose is no more than 40 g/day of the nonabsorbable composition.
  • the daily dose is no more than 30 g/day of the nonabsorbable composition.
  • the daily dose is no more than 25 g/day of the nonabsorbable composition.
  • the daily dose is no more than 20 g/day of the nonabsorbable composition.
  • the daily dose is no more than 15 g/day of the nonabsorbable composition.
  • the daily dose is no more than 10 g/day of the nonabsorbable composition.
  • the daily dose is no more than 5 g/day of the nonabsorbable composition.
  • the individual is treated with the daily dose for a period of at least one day.
  • the individual is treated with the daily dose for a period of at least one week.
  • the individual is treated with the daily dose for a period of at least one month.
  • the individual is treated with the daily dose for a period of at least two months.
  • the individual is treated with the daily dose for a period of at least three months.
  • the individual is treated with the daily dose for a period of at least several months.
  • the individual is treated with the daily dose for a period of at least six months.
  • the individual is treated with the daily dose for a period of at least one year.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 5 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 6 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 7 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 8 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 9 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 10 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 11 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 12 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 13 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 14 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 15 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 16 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 17 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 18 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 19 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 20 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 21 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 22 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 23 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 24 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 25 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 26 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 27 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 28 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 29 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 30 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 31 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 32 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 33 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 34 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 35 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 36 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 37 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 38 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 39 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 40 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 41 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 42 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 43 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 44 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 45 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 46 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 47 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 48 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 49 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has the capacity to remove at least about 50 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 5 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 6 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 7 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 8 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 9 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 11 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 12 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 13 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 14 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 15 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 16 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 17 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 18 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 19 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 20 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 21 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 22 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 23 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 24 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 25 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 26 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 27 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 28 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 29 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 30 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 31 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 32 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 33 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 34 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 35 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 36 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 37 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 38 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 39 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 40 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 41 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 42 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 43 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 44 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 45 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 46 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 47 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 48 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 49 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes at least about 50 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition removes less than 60 mEq/day of the target species.
  • the daily dose removes less than 55 mEq/day of the target species.
  • the daily dose removes less than 50 mEq/day of the target species.
  • the daily dose removes less than 45 mEq/day of the target species.
  • the daily dose removes less than 40 mEq/day of the target species.
  • the daily dose removes less than 35 mEq/day of the target species.
  • the daily dose removes less than 34 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 33 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 32 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 31 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 30 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 29 mEq/day of the target species.
  • the daily dose removes less than 28 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 27 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 26 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 25 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 24 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 23 mEq/day of the target species.
  • the daily dose removes less than 22 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 21 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 20 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 19 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 18 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 17 mEq/day of the target species.
  • the daily dose removes less than 16 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 15 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 14 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 13 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 12 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 11 mEq/day of the target species.
  • the daily dose removes less than 10 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 9 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 8 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 7 mEq/day of the target species. By way of further example, in one such embodiment the daily dose removes less than 6 mEq/day of the target species.
  • the daily dose of the nonabsorbable composition has insufficient capacity to remove more than 60 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 55 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 50 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 45 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 40 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 35 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 34 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 33 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 32 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 31 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 30 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 29 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 28 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 27 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 26 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 25 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 24 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 23 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 22 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 21 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 20 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 19 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 18 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 17 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 16 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 15 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 14 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 13 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 12 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 11 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 10 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 9 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 8 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 7 mEq/day of the target species.
  • the daily dose has insufficient capacity to remove more than 6 mEq/day of the target species.
  • the method comprises oral administration of a pharmaceutical composition to increase the individual's serum bicarbonate levels wherein: (i) the pharmaceutical composition binds a target species in the individual's digestive system when given orally, the target species being selected from the group consisting of protons, strong acids, and conjugate bases of strong acids; and (ii) the pharmaceutical composition increases the serum bicarbonate level by at least 1 mEq/l in a placebo controlled study, said increase being the difference between the cohort average serum bicarbonate level in a first cohort at the end of the study, relative to the cohort average serum bicarbonate level in a second cohort at the end of the study, wherein the first cohort's subjects receive the pharmaceutical composition and the second cohort's subjects receive a placebo, wherein the first and second cohorts each comprise at least 25 subjects, each cohort is prescribed the same diet during the study and the study lasts at least two weeks.
  • the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 100 g/day. In one embodiment, the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 50 g/day. In one embodiment, the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 30 g/day. In one embodiment, the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 25 g/day. In one embodiment, the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 20 g/day. In one embodiment, the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 15 g/day. In one embodiment, the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 10 g/day.
  • the first cohort receives a daily dose of the pharmaceutical composition that does not exceed 5 g/day.
  • the target species is protons.
  • the target species is chloride ions.
  • the target species is a strong acid.
  • the target species is HCl.
  • the pharmaceutical composition is not absorbed when ingested.
  • the individual or adult human patient has chronic kidney disease (CKD Stage 3-4; eGFR 20- ⁇ 60 ml/min/1.73 m 2 ) and a baseline serum bicarbonate value at the start of the study between 12 and 20 mEq/L.
  • the pharmaceutical composition increases the serum bicarbonate level of the the individual or adult human patient by at least 2 mEq/l in the placebo controlled study.
  • the pharmaceutical composition increases the serum bicarbonate level of the the individual or adult human patient by at least 3 mEq/l in the placebo controlled study.
  • the individual or adult human patient is not yet in need for kidney replacement therapy (dialysis or transplant).
  • the individual or adult human patient has not yet reached end stage renal disease (“ESRD”).
  • ESRD end stage renal disease
  • the individual or adult human patient has a mGFR of at least 15 mL/min/1.73 m 2 . In one embodiment, the individual or adult human patient has an eGFR of at least 15 mL/min/1.73 m 2 . In one embodiment, the individual or adult human patient has a mGFR of at least 30 mL/min/1.73 m 2 . In one embodiment, the individual or adult human patient has an eGFR of at least 30 mL/min/1.73 m 2 . In one embodiment, the individual or adult human patient has a mGFR of less than 45 mL/min/1.73 m 2 for at least three months.
  • the individual or adult human patient has an eGFR of less than 45 mL/min/1.73 m 2 for at least three months. In one embodiment, the individual or adult human patient has a mGFR of less than 60 mL/min/1.73 m 2 for at least three months. In one embodiment, the individual or adult human patient has an eGFR of less than 60 mL/min/1.73 m 2 for at least three months. In one embodiment, the individual or adult human patient has Stage 3A CKD, Stage 3B CKD, or Stage 4 CKD.
  • a further aspect of the disclosure include the methods disclosed herein in which the dose is administered less frequently than once per day (while still being administered on a regular basis).
  • the daily dose specified may, instead, be administrated on a less frequent basis.
  • the doses disclosed here may be administered once every two or three days.
  • the doses disclosed here may be administered once, twice or three times a week.
  • biomarkers of acid-base imbalance may be used as a measure of acid-base status.
  • blood serum or plasma
  • anion gap e.g., sodium, potassium, calcium, magnesium, chloride and/or sulfate
  • concentration of other electrolytes e.g., sodium, potassium, calcium, magnesium, chloride and/or sulfate
  • net acid excretion (“NAE”) urine pH, urine ammonium concentration, and/or the concentration of other electrolytes in the urine (e.g., sodium, potassium, calcium, magnesium, chloride and/or sulfate) may be used as an indicator of acid-base imbalance.
  • NAE net acid excretion
  • urine pH urine ammonium concentration
  • concentration of other electrolytes in the urine e.g., sodium, potassium, calcium, magnesium, chloride and/or sulfate
  • UAG UAG
  • treatment of an individual as described herein may improve an individuals' serum anion gap.
  • treating an acid base imbalance with a a neutral composition having the capacity to bind both protons and anions can increase serum bicarbonate without an accompanying increase in sodium or potassium (see Example 3 and FIGS. 13A, 13C and 13D ). Consequently, the serum anion gap may be improved (decreased) by at least 1 mEq/l or more (e.g., at least 2 mEq/l) within a period as short as 2 weeks (see Example 3).
  • the various aspects and embodiments may have a range of advantages, such as improved or successful treatment of metabolic acidosis. Such improvements may also include reduced side effects, increased patient compliance, reduced drug loads, increased speed of treatment, increased magnitude of treatment, avoiding unwanted changes to other electrolytes and/or reduced drug-drug interactions. A further improvement may include reducing a patient's anion gap (as defined above) as part of the methods and other aspects disclosed herein. Further useful features of the disclosed aspects can be found in the examples.
  • one aspect disclosed here is a composition for use in a method of treating metabolic acidosis in an adult human patient wherein in said treatment 0.1-12 g of said composition is administered to the patient per day, said composition being a nonabsorbable composition having the capacity to remove protons from the patient, wherein the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 2.5 mEq/g in a Simulated Small Intestine Inorganic (“SIB”) assay.
  • SIB Simulated Small Intestine Inorganic
  • compositions with this specified level of chloride binding in the “SIB” assay can be used in the specified dose range to successfully treat metabolic acidosis in adult humans.
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • This aspect is based on the data in the examples showing the absorption and removal of HCl to successfully treat patients using a composition according to this aspect, allowing the amount of the composition to be set based on its capacity to bind chloride in the SIB assay. Surprisingly, the amounts required for successful treatment were relatively low.
  • compositions for use in a method of treating metabolic acidosis in an adult human patient by increasing that patient's serum bicarbonate value by at least 1 mEq/L over 15 days of treatment said composition being a nonabsorbable composition having the capacity to remove protons from the patient.
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • This aspect is based on the data in the examples showing the absorption and removal of HCl to successfully treat patients using a composition according to this aspect which provides new detail regarding the reductions possible using a composition of the disclosure.
  • This aspect includes surprisingly rapid increases in the patient's serum bicarbonate level, for example in the first few days, as well as surprisingly large increases in serum bicarbonate level.
  • compositions for use in a method of treating metabolic acidosis in an adult human patient said patient having a serum bicarbonate level of less than 20 mEq/L prior to treatment, said composition being a nonabsorbable composition having the capacity to remove protons from the patient.
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • This aspect is based on the data in the examples showing, for the first time, the successful treatment of patients with a low serum bicarbonate level, for example levels that have not been shown to be so readily treated previously.
  • the patients with lower serum bicarbonate levels responded particularly well to the treatment and this improvement for this subgroup is one advantage of this aspect.
  • SIB Simulated Small Intestine Inorganic Buffer
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • SIB Simulated Small Intestine Inorganic Buffer
  • the composition may be administered orally, and so would be an orally administered nonabsorbable composition as defined herein.
  • composition refers to the active pharmaceutical ingredient, including any counter ions, but not to excipients. So, the “amount” of the composition is the amount of active pharmaceutical ingredient without including other parts of any unit dose form.
  • the amount of composition may be any amount disclosed herein in other sections within the range 0.1 g-12 g.
  • 1-11 g, 2-10 g, 3-9 g, 3-8 g, 3-7 g, 3-6 g, 3.5-5.5 g, 4-5 g, or 4.5-5 g of said polymer is administered to the patient per day, or 0.5 g, 1 g, 1.5 g, 2 g, 2.5 g, 3 g, 3.5 g, 4.0 g, 4.5 g or 5.0 g of the composition is administered to the patient per day.
  • the chloride ion binding capacity in a Simulated Small Intestine Inorganic Buffer (“SIB”) assay may be greater than 3, 3.5, 4, or 4.5 mEq/g.
  • SIB Simulated Small Intestine Inorganic Buffer
  • One upper limit for the chloride ion binding capacity in a SIB assay is 10 mEq/g.
  • the upper limits may be 5, 5.5, 6, 6.5, 7, 7.5, 8, 8.5, 9, 9.5 or 10 mEq/g, or there may be no upper limit specified.
  • the composition has a chloride ion binding capacity in a SIB assay is of at least 4.5 mEq/g and only 0.1-6 gs of composition is administered in the method of treating metabolic acidosis.
  • composition in these aspects can additionally have any of the properties or features specified elsewhere herein.
  • the composition may be a nonabsorbable composition as described in the following section.
  • the methods of treatment specified in these aspects may include any of the features disclosed in the preceding section regarding certain methods of treatment.
  • nonabsorbable compositions having the medical uses described herein possess the capacity to remove clinically significant quantities of one or more target species: (i) protons, (ii) the conjugate base(s) of one or more strong acids (e.g., chloride, bisulfate (HSO 4 ⁇ ) and/or sulfate (SO 4 ⁇ ) ions) and/or (iii) one or more strong acids (e.g., HCl and/or H 2 SO 4 ).
  • strong acids e.g., chloride, bisulfate (HSO 4 ⁇ ) and/or sulfate (SO 4 ⁇ ) ions
  • one or more strong acids e.g., HCl and/or H 2 SO 4
  • the nonabsorbable compositions may be selected from the group consisting of cation exchange compositions, anion exchange compositions, amphoteric ion exchange compositions, neutral compositions having the capacity to bind both protons and anions, composites thereof and mixtures thereof.
  • the nonabsorbable composition has a preferred particle size range that is (i) large enough to avoid passive or active absorption through the GI tract and (ii) small enough to not cause grittiness or unpleasant mouth feel when ingested as a powder, sachet and/or chewable tablet/dosage form with a mean particle size of at least 3 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of 5 to 1,000 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of 5 to 500 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of to 400 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of 10 to 300 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of 20 to 250 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of 30 to 250 microns.
  • the nonabsorbable composition comprises a population of particles having a mean particle size (volume distribution) in the range of 40 to 180 microns.
  • less than 7% of the particles in the population (volume distribution) have a diameter less than 10 microns.
  • less than 5% of the particles in the particles in the population (volume distribution) have a diameter less than 10 microns.
  • less than 2.5% of the particles in the particles in the population (volume distribution) have a diameter less than 10 microns.
  • less than 1% of the particles in the particles in the population (volume distribution) have a diameter less than 10 microns.
  • the particle size may be measured using the protocol set out in the abbreviations and definitions section (above).
  • a low Swelling Ratio of the nonabsorbable composition is preferred (0.5 to 10 times its own weight in water).
  • the nonabsorbable composition has a Swelling Ratio of less than 9.
  • the nonabsorbable composition has a Swelling Ratio of less than 8.
  • the nonabsorbable composition has a Swelling Ratio of less than 7.
  • the nonabsorbable composition has a Swelling Ratio of less than 6.
  • the nonabsorbable composition has a Swelling Ratio of less than 5.
  • the nonabsorbable composition has a Swelling Ratio of less than 4.
  • the nonabsorbable composition has a Swelling Ratio of less than 3.
  • the nonabsorbable composition has a Swelling Ratio of less than 2.
  • the amount of the target species (proton, conjugate base of a strong acid and/or strong acid) that is bound as the nonabsorbable composition transits the GI tract is largely a function of the binding capacity of the composition for the target species (protons, the conjugate base of a strong acid, and/or a strong acid) and the quantity of the nonabsorbable composition administered per day as a daily dose.
  • the theoretical binding capacity for a target species may be determined using a SGF assay and determining the amount of a species that appeared in or disappeared from the SGF buffer during the SGF assay.
  • the theoretical proton binding capacity of a cation exchange resin may be determined by measuring the increase in the amount of cations (other than protons) in the buffer during a SGF assay.
  • the theoretical anion binding capacity of an anion exchange resin in a form other than the chloride form
  • the theoretical anion binding capacity of a neutral composition for protons and the conjugate base of a strong acid may be determined by measuring the decrease in chloride concentration in the buffer during a SGF assay.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 0.5 mEq/g (as determined in an SGF assay).
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 1 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 2 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 3 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 4 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 5 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 7.5 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 10 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 12.5 mEq/g. By way of further example, in some embodiments the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 15 mEq/g. By way of further example, in some embodiments the nonabsorbable composition will have a theoretical binding capacity for the target species of at least about 20 mEq/g. In general, the nonabsorbable composition will typically have a theoretical binding capacity for the target species that is not in excess of about 35 mEq/g.
  • the theoretical binding capacity of the nonabsorbable compositions for the target species that is not be excess of 30 mEq/g.
  • the theoretical binding capacity of the nonabsorbable compositions for the target species may range from 2 to 25 mEq/g, 3 to 25 mEq/g, 5 to 25 mEq/g, 10 to 25 mEq/g, 5 to 20 mEq/g, 6 to mEq/g, 7.5 to 20 mEq/g, or even 10 to 20 mEq/g.
  • the binding capacities recited in this paragraph are the theoretical binding capacities for protons and the theoretical binding capacities for the conjugate base(s), independently and individually, and not the sum thereof.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 0.5 mEq/g (as determined in an SGF assay).
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 1 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 2 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 3 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 4 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 5 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 7.5 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 10 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 12.5 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 15 mEq/g.
  • the nonabsorbable composition will have a theoretical binding capacity for protons of at least about 20 mEq/g.
  • the nonabsorbable composition will typically have a theoretical binding capacity for protons that is not in excess of about 35 mEq/g.
  • the theoretical binding capacity of the nonabsorbable compositions for protons may range from 2 to 25 mEq/g, 3 to 25 mEq/g, 5 to 25 mEq/g, 10 to 25 mEq/g, 5 to 20 mEq/g, 6 to mEq/g, 7.5 to 20 mEq/g, or even 10 to 20 mEq/g.
  • the binding capacities recited in this paragraph are the theoretical binding capacities for protons and the theoretical binding capacities for the conjugate base(s), independently and individually, and not the sum thereof.
  • Phosphate, bicarbonate, bicarbonate equivalents, the conjugate bases of bile and fatty acids are potential interfering anions for chloride or other conjugate bases of strong acids (e.g., HSO 4 ⁇ and SO 4 2 ⁇ ) in the stomach and small intestine. Therefore, rapid and preferential binding of chloride over phosphate, bicarbonate equivalents, and the conjugate bases of bile and fatty acids in the small intestine is desirable and the SIB assay may be used to determine kinetics and preferential binding.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 1 mEq/g in a Simulated Small Intestine Inorganic Buffer (“SIB”) assay.
  • SIB Simulated Small Intestine Inorganic Buffer
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 1.5 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 2 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 2.5 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 3 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 3.5 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 4 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 4.5 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 5 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 5.5 mEq/g in a SIB assay.
  • the nonabsorbable composition is characterized by a chloride ion binding capacity of at least 6 mEq/g in a SIB assay.
  • the nonabsorbable composition binds a significant amount of chloride relative to phosphate as exhibited, for example, in a SIB assay.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.1:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.2:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.25:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.3:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.35:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.4:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.45:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.5:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 2:3, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.75:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 0.9:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 1:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 1.25:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 1.5:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 1.75:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 2:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 2.25:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 2.5:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 2.75:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 3:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 4:1, respectively.
  • the ratio of the amount of bound chloride to bound phosphate in a SIB assay is at least 5:1, respectively.
  • the orally administered nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in Simulated Gastric Fluid of at least 1 mEq/g in a SGF assay.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 2 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 3 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 4 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 5 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 6 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 7 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 8 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 9 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 10 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 11 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 12 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 13 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity in a SGF assay of at least 14 mEq/g.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity after 1 hour in SGF that is at least 50% of the proton-binding capacity and the chloride binding capacity, respectively, of the nonabsorbable composition at 24 hours in SGF.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity after 1 hour in SGF that is at least 60% of the proton-binding capacity and the chloride binding capacity, respectively, of the nonabsorbable composition at 24 hours in SGF.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity after 1 hour in SGF that is at least 70% of the proton-binding capacity and the chloride binding capacity, respectively, of the nonabsorbable composition at 24 hours in SGF.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity after 1 hour in SGF that is at least 80% of the proton-binding capacity and the chloride binding capacity, respectively, of the nonabsorbable composition at 24 hours in SGF.
  • the nonabsorbable composition is characterized by a proton-binding capacity and a chloride binding capacity after 1 hour in SGF that is at least 90% of the proton-binding capacity and the chloride binding capacity, respectively, of the nonabsorbable composition at 24 hours in SGF.
  • the nonabsorbable composition is a cation exchange material comprising an insoluble (in the gastric environment) support structure and exchangeable cations.
  • the cation exchange material may be organic (e.g., polymeric), inorganic (e.g., a zeolite) or a composite thereof.
  • the exchangeable cations may be selected, for example, from the group consisting of lithium, sodium, potassium, calcium, magnesium, iron and combinations thereof, and more preferably from the group consisting of sodium, potassium, calcium, magnesium, and combinations thereof.
  • the nonabsorbable composition contain a combination of exchangeable cations that establish or maintain electrolyte homeostasis.
  • the nonabsorbable composition optionally contains exchangeable sodium ions, but when included, the amount of the sodium ions in a daily dose is insufficient to increase the patient's serum sodium ion concentration to a value outside the range of 135 to 145 mEq/l.
  • the nonabsorbable composition optionally contains exchangeable potassium ions, but when included, the amount of the potassium ions in a daily dose is insufficient to increase the patient's serum potassium ion concentration to a value outside the range of 3.7 to 5.2 mEq/L.
  • the nonabsorbable composition optionally contains exchangeable magnesium ions, but when included, the amount of the magnesium ions in a daily dose is insufficient to increase the patient's serum magnesium ion concentration to a value outside the range of 1.7 to 2.2 mg/dL.
  • the nonabsorbable composition optionally contains exchangeable calcium ions, but when included, the amount of the calcium ions in a daily dose is insufficient to increase the patient's serum calcium ion concentration to a value outside the range of 8.5 to 10.2 mg/dL.
  • the nonabsorbable composition contains a combination of exchangeable cations selected from the group consisting of sodium, potassium, calcium, magnesium, and combinations thereof, designed to maintain serum Na + levels within the range of 135 to 145 mEq/l, serum K + levels within the range of 3.7 to 5.2 mEq/L, serum Mg 2+ levels within the range of 1.7 to 2.2 mg/dL and serum Ca 2+ levels within the range of 8.5 to 10.2 mg/dL.
  • exchangeable cations selected from the group consisting of sodium, potassium, calcium, magnesium, and combinations thereof, designed to maintain serum Na + levels within the range of 135 to 145 mEq/l, serum K + levels within the range of 3.7 to 5.2 mEq/L, serum Mg 2+ levels within the range of 1.7 to 2.2 mg/dL and serum Ca 2+ levels within the range of 8.5 to 10.2 mg/dL.
  • the nonabsorbable composition is a cation exchange material comprising an insoluble (in the gastric environment) support structure, optionally containing exchangeable sodium ions cations.
  • the cation exchange material may be organic (e.g., polymeric), inorganic (e.g., a molecular sieve) or a composite thereof.
  • the nonabsorbable composition contains less than 12% by weight sodium.
  • the nonabsorbable composition contains less than 9% by weight sodium.
  • the nonabsorbable composition contains less than 6% by weight sodium.
  • the nonabsorbable composition contains less than 3% by weight sodium.
  • the nonabsorbable composition contains less than 1% by weight sodium. By way of further example, in one such embodiment the nonabsorbable composition contains less than 0.1% by weight sodium. By way of further example, in one such embodiment the nonabsorbable composition contains less than 0.01% by weight sodium. By way of further example, in one such embodiment the nonabsorbable composition contains between 0.05 and 3% by weight sodium.
  • the nonabsorbable composition is a resin comprising any of a wide range of crosslinked polymeric materials that are able to bind protons in aqueous solutions.
  • exemplary crosslinked polymeric material comprises a polyanion crosslinked material selected from poly(carboxylic acids), poly(acrylic acids), poly(sulfonic acids), poly(maleic acids), poly(phenols), functionalized polyols and poly(alcohols), poly(hydroxamic acids), poly(imides) and copolymers thereof.
  • the polyanion is coordinated to exchangeable monovalent cations, divalent cations, or a combination thereof.
  • Exemplary monovalent cations include lithium, sodium, and potassium, or any combination thereof.
  • Exemplary divalent cations include magnesium and calcium or combinations thereof.
  • the nonabsorbable composition is a cation exchange resin comprising a polyanion backbone that exchanges cations for protons and has an average pKa of at least 4.
  • the polyanion backbone has an average pKa of 4-5.
  • the polyanion backbone has an average pKa of 5-6.
  • the polyanion backbone has an average pKa of 6-7.
  • the polyanion backbone has an average pKa of greater than 7.
  • Exemplary cation exchange resins include poly(carboxylic acids), poly(acrylic acids), poly(sulfonic acids), poly(maleic acids), poly(phenols), functionalized polyols and poly(alcohols), poly(hydroxamic acids), poly(imides) and copolymers thereof.
  • these polyanion backbones are further functionalized with functional groups to affect the pKa. These functional groups can increase pKa when electron donating, or decrease pKa when electron withdrawing.
  • Exemplary electron donating groups include amino, hydroxyl, methyl ether, ether, phenyl, and amido.
  • Exemplary electron withdrawing groups include flouro, chloro, halo, sulphonyl, nitroxyl, trifluoromethyl, and cyano.
  • Further exemplary cation exchange resins include resins modified with protonable functional groups including carboxylic acids and functionalized alcohols.
  • Polymeric cation exchanger resins may be prepared using a range of chemistries, including for example, (i) substitution polymerization of polyfunctional reagents at least one of which comprises basic anionic or conjugate-acid moieties, (2) radical polymerization of a monomer comprising at least one acid or conjugate-acid containing moiety, and (3) crosslinking of a basic anionic or conjugate-acid containing intermediate with a polyfunctional crosslinker, optionally containing basic anionic or conjugate-acid moieties.
  • the resulting crosslinked polymers may thus, for example, be crosslinked homopolymers or crosslinked copolymers.
  • the resulting crosslinked polymers will typically possess repeat units comprising basic anionic or conjugate-acid, separated by the same or varying lengths of repeating linker (or intervening) units.
  • the polymers comprise repeat units comprising a basic anionic or conjugate-acid moiety and an intervening linker unit.
  • multiple basic anionic or conjugate-acid containing repeat units are separated by one or more linker units.
  • the polyfunctional crosslinkers may comprise proton binding functional groups, e.g. basic anionic, (“active crosslinkers”) or may lack proton binding functional groups such as acrylates (“passive crosslinkers”).
  • a basic anion or conjugate-acid monomer is polymerized and the polymer is concurrently crosslinked in a substitution polymerization reaction.
  • the basic anion or conjugate-acid reactant (monomer) in the concurrent polymerization and crosslinking reaction can react more than one time for the substitution polymerization.
  • the basic anion or conjugate-acid monomer is a branched basic anion or conjugate-acid possessing at least two reactive moieties to participate in the substitution polymerization reaction.
  • the nonabsorbable composition comprises a cation exchange ceramic material.
  • Porous inorganic binders exhibit a range of properties. Functionally, they are able to sequester materials on the basis of their size and polarity, as they exhibit a framework charge with porous structure. They are structurally diverse and can be crystalline or non-crystalline crystalline (amorphous). Classes of porous materials that fall under the class of inorganic binders include hydrous oxides (e.g., aluminum oxide) and metal alumino-silicate compounds where the metal can be an alkali or alkali earth metal such sodium, potassium, lithium, magnesium or calcium. Many of these compounds have well-defined crystalline structures. This class of compounds has been used for various biopharmaceutical applications.
  • the pore diameters of inorganic microporous and mesoporous materials are measured in ⁇ ngströms ( ⁇ ) or nanometers (nm). According to IUPAC notation, microporous materials have pore diameters of less than 2 nm (20 ⁇ ) and macroporous materials have pore diameters of greater than 50 nm (500 ⁇ ); the mesoporous category thus lies in the middle with pore diameters between 2 and 50 nm (20-500 ⁇ ).
  • the porosity of inorganic porous materials can be tuned or designed, by the appropriate use of poragen or “co-monomer metals” within the lattices of the porous material.
  • the pore size has been seen to range in size from 3 ⁇ to 8 ⁇ .
  • These compositions have a porous system allowing solute together with other dissolved species to enter the porous framework of the material, resulting in absorption of the the dissolved species.
  • Tuning the cavities and pore size of the materials can allow adsorption of molecules of particular dimensions, while rejecting those of larger dimensions.
  • the chloride ion has the advantage of its small size (the radius of chloride anion is 1.8 ⁇ , and the molecular weight of chloride anion is 35.5) compared to the other species present in the digestive tract.
  • the nonabsorbable composition comprises a molecular sieve, such as a molecular sieve selected from the group consisting of silica, titanosilicate, metalloaluminate, aluminophosphate and gallogerminate molecular sieves.
  • the nonabsorbable composition comprises a zeolite, a borosilicate, a gallosilicate, a ferrisilicate or a chromosilicate molecular sieve.
  • Inorganic porous materials exhibit the property of sequestering substances from an external environment.
  • the mechanism to bind proton or chloride or HCl can be either an adsorptive or absorptive mechanism, where the ions are bound via the specific porosity of the matrix, or an ion exchange mechanism.
  • the strong adsorptive force in zeolite molecular sieves are due to the polarity of the surface (hydroxyl metalloid) and cations that are exposed within the crystal lattice.
  • the cations on the surface act as a site of strong localized positive charge that electrostatically attract the partial negative charges of polar molecules (for example, the chloride of HCl).
  • a basic formula for zeolite can be represented by, M 2/n O.Al 2 O 3 .xSiO 2 .yH 2 O where M is a cation of n valence.
  • the fundamental building block of the molecular sieve structure is tetrahedral with 4 oxygen anions surrounding a silicon or alumina cation.
  • Sodium ions or other cations e.g. potassium, calcium
  • the sodium can be exchanged or the sodium can function as a permanent positive charge within the crystal lattice thus providing the electrostatic interaction.
  • hydrochloric acid can be sequestered from solution via a cation exchange mechanism (sodium for proton), anion exchange mechanism (hydroxide for chloride), or via electrostatic interaction of the hydrochloric acid ionic species.
  • the methods used to bind HCl are well known in the art and involve contacting the molecular sieve with a solution containing the desired HCl concentration in water.
  • Exchange conditions include a temperature of about 25° C. to about 100° C., and a time of about 20 minutes to about 2 hours. These conditions include conditions and exposure times encountered in the gastrointestinal tract.
  • the nonabsorbable composition is an anion exchange material comprising an insoluble (in the gastric environment) support structure and exchangeable anions.
  • the anion exchange material may be organic (e.g., polymeric), inorganic (e.g., an apatite, hydrotalcite or a hydrated gel of aluminum, iron(III) or zirconium hydroxide) or a composite thereof.
  • the nonabsorbable composition comprises an anion exchange material.
  • anion exchange materials include strongly and weakly basic anion exchange materials.
  • the anion exchange material may include any of a wide range of polymers comprising quaternary amine moieties, phosphonium salts, N-heteroaromatic salts, or combinations thereof.
  • Other exemplary anion exchange materials include poly(ionic liquids), wherein the side chain is selected from the group consisting of salts of tetraalkyl ammonium, imidazolium, pyridinium, pyrrolidonium, guanidinium, piperidinium, and tetraalkyl phosphonium cations and combinations thereof.
  • the anion exchange material is a halide responsive polymer such that a conformational change occurs when about 1 mEq/g to about 35 mEq/g of chloride is initially bound to the polymer and subsequently retained for the duration of the GI transit time.
  • the halide response conformational change occurs when 2 mEq/g to about 25 mEq/g chloride is bound, and in certain more specific embodiments, the halide response conformational change occurs when 3 to 25 mEq/g, 5 to 25 mEq/g, 10 to 25 mEq/g, 5 to 20 mEq/g, 6 to 20 mEq/g, 7.5 to 20 mEq/g, or even 10 to 20 mEq/g chloride is bound.
  • the polymeric backbone of any of the aforementioned polymers can derive from vinyl, allyl, styrenic, acrylamide, meth(acrylamide), or copolymers thereof.
  • the anion exchange functionality may be incorporated into the backbone of the polymer.
  • examples include poly(tetraalkyl ammonium), poly(imidazolium), poly(pyridinium), poly(pyrrolidonium), poly(piperidinium), and poly(tetraalkyl phosphonium) cations or combinations thereof.
  • the exchangeable anion can consist of hydroxide, bicarbonate, acetate, nitrate or any pharmaceutically and biologically acceptable base or combination thereof.
  • the nonabsorbable composition is an anion exchange material comprising at least 1 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion, or a combination thereof.
  • the nonabsorbable composition has the capacity to induce an increase in the individual's serum bicarbonate value, at least in part, by delivering a physiologically significant amount of hydroxide, carbonate, citrate or other bicarbonate equivalent, or a combination thereof.
  • Exemplary bicarbonate equivalent anions include acetate, lactate and the conjugate bases of other short chain carboxylic acids.
  • the nonabsorbable composition comprises at least 2 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises at least 3 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises at least 4 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises at least 5 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition is an anion exchange material comprising less than 10 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion, or a combination thereof. In one such embodiment, the nonabsorbable composition comprises less than 7.5 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion. By way of further example, in one such embodiment the nonabsorbable composition comprises less than 5 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises less than 2.5 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises less than 1 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises less than 0.1 mEq/g of an anion selected from the group consisting of hydroxide, carbonate, citrate or other bicarbonate equivalent anion.
  • the nonabsorbable composition comprises an amphoteric ion exchange resin.
  • amphoteric ion-exchange resins include crosslinked polystyrene, polyethylene or the like as a base material and quaternary ammonium group, carboxylic acid group and the like in (i) the same pendant groups (e.g., betaine-containing pendant groups) such as the amphoteric resin sold under the trade designation DIAION AMP03 (Mitsubishi Chemical Corporation) or (ii) different pendant groups (e.g., mixed charged copolymers containing the residues of at least two different monomers, one containing ammonium groups and one containing carboxylic acid groups), to provide a function of ion-exchanging the both of cations and negative ions.
  • DIAION AMP03 Mitsubishi Chemical Corporation
  • Exemplary amphoteric ion-exchange resins containing a mixture of cation and anion exchange sites also include resins in which a linear polymer is trapped inside a crosslinked ion exchange resin, such as the amphoteric resin sold under the trade designation DOWEXTM Retardion 11A8 (Dow Chemical Company).
  • the nonabsorbable composition comprises a neutral composition having the capacity to bind both protons and anions.
  • exemplary neutral nonabsorbable compositions that bind both protons and anions include polymers functionalized with propylene oxide, polymers functionalized with Michael acceptors, expanded porphyrins, covalent organic frameworks, and polymers containing amine and/or phosphine functional groups.
  • the nonabsorbable composition binds chloride ions
  • the nonabsorbable composition selectively bind chloride ions relative to other counter ions such as bicarbonate equivalent anions, phosphate anions, and the conjugate bases of bile and fatty acids.
  • the nonabsorbable composition (i) remove more chloride ions than bicarbonate equivalent anions (ii) remove more chloride ions than phosphate anions, and (iii) remove more chloride ions than the conjugate bases of bile and fatty acids.
  • treatment with the nonabsorbable composition does not induce or exacerbate hypophosphatemia (i.e., a serum phosphorous concentration of less than about 2.4 mg/dL, does not significantly elevate low density lipoproteins (“LDL”), or otherwise negatively impact serum or colon levels of metabolically relevant anions.
  • hypophosphatemia i.e., a serum phosphorous concentration of less than about 2.4 mg/dL
  • LDL low density lipoproteins
  • the pharmaceutical composition comprises a crosslinked polymer containing the residue of an amine corresponding to Formula 1:
  • R 1 , R 2 and R 3 are independently hydrogen, hydrocarbyl, substituted hydrocarbyl provided, however, at least one of R 1 , R 2 and R 3 is other than hydrogen. Stated differently, at least one of R 1 , R 2 and R 3 is hydrocarbyl or substituted hydrocarbyl, and the others of R 1 , R 2 and R 3 are independently hydrogen, hydrocarbyl, or substituted hydrocarbyl. In one embodiment, for example, R 1 , R 2 and R 3 are independently hydrogen, aryl, aliphatic, heteroaryl, or heteroaliphatic provided, however, each of R 1 , R 2 and R 3 are not hydrogen.
  • R 1 , R 2 and R 3 are independently hydrogen, saturated hydrocarbons, unsaturated aliphatic, unsaturated heteroaliphatic, heteroalkyl, heterocyclic, aryl or heteroaryl, provided, however, each of R 1 , R 2 and R 3 are not hydrogen.
  • R 1 , R 2 and R 3 are independently hydrogen, alkyl, alkenyl, allyl, vinyl, aryl, aminoalkyl, alkanol, haloalkyl, hydroxyalkyl, ethereal, heteroaryl or heterocyclic provided, however, each of R 1 , R 2 and R 3 are not hydrogen.
  • R 1 , R 2 and R 3 are independently hydrogen, alkyl, aminoalkyl, alkanol, aryl, haloalkyl, hydroxyalkyl, ethereal, heteroaryl or heterocyclic provided, however, each of R 1 , R 2 and R 3 are not hydrogen.
  • R 1 and R 2 in combination with the nitrogen atom to which they are attached together constitute part of a ring structure, so that the monomer as described by Formula 1 is a nitrogen-containing heterocycle (e.g., piperidine) and R 3 is hydrogen, or heteroaliphatic.
  • R 1 , R 2 and R 3 are independently hydrogen, aliphatic or heteroaliphatic provided, however, at least one of R 1 , R 2 and R 3 is other than hydrogen.
  • R 1 , R 2 and R 3 are independently hydrogen, allyl, or aminoalkyl.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 1 wherein R 1 , R 2 , and R 3 are independently hydrogen, heteroaryl, aryl, aliphatic or heteroaliphatic provided, however, at least one of R 1 , R 2 , and R 3 is aryl or heteroaryl.
  • R 1 and R 2 in combination with the nitrogen atom to which they are attached, may form a saturated or unsaturated nitrogen-containing heterocyclic ring.
  • R, and R 2 in combination with the nitrogen atom to which they are attached may constitute part of a pyrrolidino, pyrole, pyrazolidine, pyrazole, imidazolidine, imidazole, piperidine, pyridine, piperazine, diazine, or triazine ring structure.
  • R 1 and R 2 in combination with the nitrogen atom to which they are attached may constitute part of a piperidine ring structure.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 1 wherein R 1 , R 2 , and R 3 are independently hydrogen, aliphatic, or heteroaliphatic provided, however, at least one of R 1 , R 2 , and R 3 is other than hydrogen.
  • R 1 , R 2 , and R 3 may independently be hydrogen, alkyl, alkenyl, allyl, vinyl, aminoalkyl, alkanol, haloalkyl, hydroxyalkyl, ethereal, or heterocyclic provided, however, at least one of R 1 , R 2 , and R 3 is other than hydrogen.
  • R 1 and R 2 in combination with the nitrogen atom to which they are attached, may form a saturated or unsaturated nitrogen-containing heterocyclic ring.
  • R 1 and R 2 in combination with the nitrogen atom to which they are attached may constitute part of a pyrrolidino, pyrole, pyrazolidine, pyrazole, imidazolidine, imidazole, piperidine, piperazine, or diazine ring structure.
  • R 1 and R 2 in combination with the nitrogen atom to which they are attached may constitute part of a piperidine ring structure.
  • the amine corresponding to Formula 1 is acyclic and at least one of R 1 , R 2 , and R 3 is aliphatic or heteroaliphatic.
  • R 1 , R 2 , and R 3 are independently hydrogen, alkyl, allyl, vinyl, alicyclic, aminoalkyl, alkanol, or heterocyclic, provided at least one of R 1 , R 2 , and R 3 is other than hydrogen.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 1 and the crosslinked polymer is prepared by substitution polymerization of the amine corresponding to Formula 1 with a polyfunctional crosslinker (optionally also comprising amine moieties) wherein R 1 , R 2 , and R 3 are independently hydrogen, alkyl, aminoalkyl, or alkanol, provided at least one of R 1 , R 2 , and R 3 is other than hydrogen.
  • a polyfunctional crosslinker optionally also comprising amine moieties
  • the molecular weight per nitrogen of the polymers of the present disclosure may range from about 40 to about 1000 Daltons. In one embodiment, the molecular weight per nitrogen of the polymer is from about 40 to about 500 Daltons. In another embodiment, the molecular weight per nitrogen of the polymer is from about 50 to about 170 Daltons. In another embodiment, the molecular weight per nitrogen of the polymer is from about 60 to about 110 Daltons.
  • an amine-containing monomer is polymerized and the polymer is concurrently crosslinked in a substitution polymerization reaction in the first reaction step.
  • the amine reactant (monomer) in the concurrent polymerization and crosslinking reaction can react more than one time for the substitution polymerization.
  • the amine monomer is a linear amine possessing at least two reactive amine moieties to participate in the substitution polymerization reaction.
  • the amine monomer is a branched amine possessing at least two reactive amine moieties to participate in the substitution polymerization reaction.
  • Crosslinkers for the concurrent substitution polymerization and crosslinking typically have at least two amine-reactive moieties such as alkyl-chlorides, and alkyl-epoxides.
  • primary amines react at least once and potentially may react up to three times with the crosslinker
  • secondary amines can react up to twice with the crosslinkers
  • tertiary amines can only react once with the crosslinker.
  • the formation of a significant number of quaternary nitrogens/amines is generally not preferred because quaternary amines cannot bind protons.
  • Exemplary amines that may be used in substitution polymerization reactions described herein include 1,3-Bis[bis(2-aminoethyl)amino]propane, 3-Amino-1- ⁇ [2-(bis ⁇ 2-[bis(3-aminopropyl)amino]ethyl ⁇ amino)ethyl](3-aminopropyl)amino ⁇ propane, 2-[Bis(2-aminoethyl)amino]ethanamine, Tris(3-aminopropyl)amine, 1,4-Bis[bis(3-aminopropyl)amino]butane, 1,2-Ethanediamine, 2-Amino-1-(2-aminoethylamino)ethane, 1,2-Bis(2-aminoethylamino)ethane, 1,3-Propanediamine, 3,3′-Diaminodipropylamine, 2,2-dimethyl-1,3-propanediamine, 2-methyl-1
  • crosslinking agents that may be used in substitution polymerization reactions and post-polymerization crosslinking reactions include, but are not limited to, one or more multifunctional crosslinking agents such as: dihaloalkanes, haloalkyloxiranes, alkyloxirane sulfonates, di(haloalkyl)amines, tri(haloalkyl) amines, diepoxides, triepoxides, tetraepoxides, bis (halomethyl)benzenes, tri(halomethyl)benzenes, tetra(halomethyl)benzenes, epihalohydrins such as epichlorohydrin and epibromohydrin poly(epichlorohydrin), (iodomethyl)oxirane, glycidyl tosylate, glycidyl 3-nitrobenzenesulfonate, 4-tosyloxy-1,2-epoxybutane, bromo-1,2-epoxy
  • the carbon to nitrogen ratio of the polymers of the present disclosure may range from about 2:1 to about 6:1, respectively.
  • the carbon to nitrogen ratio of the polymers of the present disclosure may range from about 2.5:1 to about 5:1, respectively.
  • the carbon to nitrogen ratio of the polymers of the present disclosure may range from about 3:1 to about 4.5:1, respectively.
  • the carbon to nitrogen ratio of the polymers of the present disclosure may range from about 3.25:1 to about 4.25:1, respectively.
  • the carbon to nitrogen ratio of the polymers of the present disclosure may range from about 3.4:1 to about 4:1, respectively.
  • the molecular weight per nitrogen of the polymer is from about 60 to about 110 Daltons.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 1a and the crosslinked polymer is prepared by radical polymerization of an amine corresponding to Formula 1a:
  • R 4 and R 5 are independently hydrogen, hydrocarbyl, or substituted hydrocarbyl.
  • R 4 and R 5 are independently hydrogen, saturated hydrocarbon, unsaturated aliphatic, aryl, heteroaryl, unsaturated heteroaliphatic, heterocyclic, or heteroalkyl.
  • R 4 and R 5 are independently hydrogen, aliphatic, heteroaliphatic, aryl, or heteroaryl.
  • R 4 and R 5 are independently hydrogen, alkyl, alkenyl, allyl, vinyl, aryl, aminoalkyl, alkanol, haloalkyl, hydroxyalkyl, ethereal, heteroaryl or heterocyclic.
  • R 4 and R 5 are independently hydrogen, alkyl, allyl, aminoalkyl, alkanol, aryl, haloalkyl, hydroxyalkyl, ethereal, or heterocyclic.
  • R 4 and R 5 in combination with the nitrogen atom to which they are attached together constitute part of a ring structure, so that the monomer as described by Formula 1a is a nitrogen-containing heterocycle (e.g., piperidine).
  • R 4 and R 5 are independently hydrogen, aliphatic or heteroaliphatic.
  • R 4 and R 5 are independently hydrogen, allyl, or aminoalkyl.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 1 b and the crosslinked polymer is prepared by substitution polymerization of the amine corresponding to Formula 1b with a polyfunctional crosslinker (optionally also comprising amine moieties):
  • R 4 and R 5 are independently hydrogen, hydrocarbyl, or substituted hydrocarbyl
  • R 6 is aliphatic
  • Re and R 82 are independently hydrogen, aliphatic, or heteroaliphatic.
  • R 4 and R 5 are independently hydrogen, saturated hydrocarbon, unsaturated aliphatic, aryl, heteroaryl, heteroalkyl, or unsaturated heteroaliphatic.
  • R 4 and R 5 are independently hydrogen, aliphatic, heteroaliphatic, aryl, or heteroaryl.
  • R 4 and R 5 are independently hydrogen, alkyl, alkenyl, allyl, vinyl, aryl, aminoalkyl, alkanol, haloalkyl, hydroxyalkyl, ethereal, heteroaryl or heterocyclic.
  • R 4 and R 5 are independently hydrogen, alkyl, alkenyl, aminoalkyl, alkanol, aryl, haloalkyl, hydroxyalkyl, ethereal, heteroaryl or heterocyclic.
  • R 4 and R 5 (in combination with the nitrogen atom to which they are attached) together constitute part of a ring structure, so that the monomer as described by Formula 1a is a nitrogen-containing heterocycle (e.g., piperidine).
  • R 4 and R 5 are independently hydrogen, aliphatic or heteroaliphatic.
  • R 4 and R 5 are independently hydrogen, allyl, or aminoalkyl.
  • R 6 may be methylene, ethylene or propylene, and R 61 and R 62 may independently be hydrogen, allyl or aminoalkyl.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 1c:
  • R 7 is hydrogen, aliphatic or heteroaliphatic and R 8 is aliphatic or heteroaliphatic.
  • R 7 is hydrogen and R 8 is aliphatic or heteroaliphatic.
  • R 7 and R 8 are independently aliphatic or heteroaliphatic.
  • at least one of R 7 and R 8 comprises an allyl moiety.
  • at least one of R 7 and R 8 comprises an aminoalkyl moiety.
  • R 7 and R 8 each comprise an allyl moiety.
  • R 7 and R 8 each comprise an aminoalkyl moiety.
  • R 7 comprises an allyl moiety and R 8 comprises an aminoalkyl moiety.
  • R 7 comprises an allyl moiety and R 8 comprises an aminoalkyl moiety.
  • R 7 comprises an allyl moiety and R 8 comprises an aminoalkyl moiety.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2:
  • n and n are independently non-negative integers
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, hydrocarbyl, or substituted hydrocarbyl;
  • X 2 is hydrocarbyl or substituted hydrocarbyl
  • each X 11 is independently hydrogen, hydrocarbyl, substituted hydrocarbyl, hydroxyl, amino, boronic acid, or halo;
  • z is a non-negative number.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2, the crosslinked polymer is prepared by (i) substitution polymerization of the amine corresponding to Formula 2 with a polyfunctional crosslinker (optionally also comprising amine moieties) or (2) radical polymerization of an amine corresponding to Formula 2, and m and n are independently 0, 1, 2 or 3 and n is 0 or 1.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2
  • the crosslinked polymer is prepared by (i) substitution polymerization of the amine corresponding to Formula 2 with a polyfunctional crosslinker (optionally also comprising amine moieties) or (2) radical polymerization of an amine corresponding to Formula 2
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, aliphatic, aryl, heteroaliphatic, or heteroaryl.
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, aliphatic, or heteroaliphatic.
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, alkyl, allyl, vinyl, or aminoalkyl.
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, alkyl, allyl, vinyl, —(CH 2 ) d NH 2 , —(CH 2 ) d N[(CH 2 ) e NH 2 )] 2 where d and e are independently 2-4.
  • m and z may independently be 0, 1, 2 or 3 and n is 0 or 1.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2
  • the crosslinked polymer is prepared by (i) substitution polymerization of the amine corresponding to Formula 2 with a polyfunctional crosslinker (optionally also comprising amine moieties) or (2) radical polymerization of an amine corresponding to Formula 2
  • X 2 is aliphatic or heteroaliphatic.
  • X 2 is aliphatic or heteroaliphatic and R 10 , R 20 , R 30 , and R 40 are independently hydrogen, aliphatic, heteroaliphatic.
  • X 2 is alkyl or aminoalkyl and R 10 , R 20 , R 30 , and R 40 are independently hydrogen, aliphatic, or heteroaliphatic.
  • X 2 is alkyl or aminoalkyl and R 10 , R 20 , R 30 , and R 40 are independently hydrogen, alkyl, allyl, vinyl, or aminoalkyl.
  • m and z may independently be 0, 1, 2 or 3 and n is 0 or 1.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2, the crosslinked polymer is prepared by (i) substitution polymerization of the amine corresponding to Formula 2 with a polyfunctional crosslinker (optionally also comprising amine moieties) or (2) radical polymerization of an amine corresponding to Formula 2, and m is a positive integer.
  • m is a positive integer
  • z is zero and R 20 is hydrogen, aliphatic or heteroaliphatic.
  • m is a positive integer (e.g., 1 to 3)
  • z is a positive integer (e.g., 1 to 2)
  • X 11 is hydrogen, aliphatic or heteroaliphatic
  • R 20 is hydrogen, aliphatic or heteroaliphatic.
  • m is a positive integer
  • z is zero, one or two
  • X 11 is hydrogen alkyl, alkenyl, or aminoalkyl
  • R 20 is hydrogen, alkyl, alkenyl, or aminoalkyl.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2, the crosslinked polymer is prepared by (i) substitution polymerization of the amine corresponding to Formula 2 with a polyfunctional crosslinker (optionally also comprising amine moieties) or (2) radical polymerization of an amine corresponding to Formula 2, and n is a positive integer and R 30 is hydrogen, aliphatic or heteroaliphatic.
  • n is 0 or 1
  • R 30 is hydrogen, alkyl, alkenyl, or aminoalkyl.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2, the crosslinked polymer is prepared by (i) substitution polymerization of the amine corresponding to Formula 2 with a polyfunctional crosslinker (optionally also comprising amine moieties) or (2) radical polymerization of an amine corresponding to Formula 2, and m and n are independently non-negative integers and X 2 is aliphatic or heteroaliphatic.
  • m is 0 to 2
  • n is 0 or 1
  • X 2 is aliphatic or heteroaliphatic
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, aliphatic, or heteroaliphatic.
  • m is 0 to 2
  • n is 0 or 1
  • X 2 is alkyl or aminoalkyl
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, aliphatic, or heteroaliphatic.
  • m is 0 to 2
  • n is 0 or 1
  • X 2 is alkyl or aminoalkyl
  • R 10 , R 20 , R 30 , and R 40 are independently hydrogen, alkyl, alkenyl, or aminoalkyl.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2a and the crosslinked polymer is prepared by substitution polymerization of the amine corresponding to Formula 2a with a polyfunctional crosslinker (optionally also comprising amine moieties):
  • n and n are independently non-negative integers
  • each R 11 is independently hydrogen, hydrocarbyl, heteroaliphatic, or heteroaryl;
  • R 21 and R 31 are independently hydrogen or heteroaliphatic
  • R 41 is hydrogen, substituted hydrocarbyl, or hydrocarbyl
  • X 2 is alkyl or substituted hydrocarbyl
  • each X 12 is independently hydrogen, hydroxy, amino, aminoalkyl, boronic acid or halo;
  • z is a non-negative number.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2a
  • the crosslinked polymer is prepared by substitution polymerization of the amine corresponding to Formula 1 with a polyfunctional crosslinker (optionally also comprising amine moieties).
  • a polyfunctional crosslinker optionally also comprising amine moieties.
  • m and z are independently 0, 1, 2 or 3, and n is 0 or 1.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2a
  • the crosslinked polymer is prepared by substitution polymerization of the amine corresponding to Formula 2a with a polyfunctional crosslinker (optionally also comprising amine moieties)
  • each R 11 is independently hydrogen, aliphatic, aminoalkyl, haloalkyl, or heteroaryl
  • R 21 and R 31 are independently hydrogen or heteroaliphatic
  • R 41 is hydrogen, aliphatic, aryl, heteroaliphatic, or heteroaryl.
  • each R 11 is hydrogen, aliphatic, aminoalkyl, or haloalkyl
  • R 21 and R 31 are independently hydrogen or heteroaliphatic
  • R 41 is hydrogen, alkylamino, aminoalkyl, aliphatic, or heteroaliphatic.
  • each R 11 is hydrogen, aliphatic, aminoalkyl, or haloalkyl
  • R 21 and R 31 are hydrogen or aminoalkyl
  • R 41 is hydrogen, aliphatic, or heteroaliphatic.
  • each R 11 and R 41 is independently hydrogen, alkyl, or aminoalkyl
  • R 21 and R 31 are independently hydrogen or heteroaliphatic.
  • each R 11 and R 41 is independently hydrogen, alkyl, —(CH 2 ) d NH 2 , —(CH 2 ) d N[(CH 2 ) e NH 2 )] 2 where d and e are independently 2-4, and R 21 and R 31 are independently hydrogen or heteroaliphatic.
  • m and z may independently be 0, 1, 2 or 3, and n is 0 or 1.
  • Exemplary amines for the synthesis of polymers comprising repeat units corresponding to Formula 2a include, but are not limited to, amines appearing in Table A.
  • crosslinkers for the synthesis of polymers comprising the residue of amines corresponding to Formula 2a include but are not limited to crosslinkers appearing in Table B.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2b and the crosslinked polymer is prepared by radical polymerization of an amine corresponding to Formula 2b:
  • n and n are independently non-negative integers
  • each R 12 is independently hydrogen, substituted hydrocarbyl, or hydrocarbyl
  • R 22 and R 32 are independently hydrogen substituted hydrocarbyl, or hydrocarbyl
  • R 42 is hydrogen, hydrocarbyl or substituted hydrocarbyl
  • X 2 is alkyl, aminoalkyl, or alkanol
  • each X 13 is independently hydrogen, hydroxy, alicyclic, amino, aminoalkyl, halogen, alkyl, heteroaryl, boronic acid or aryl;
  • z is a non-negative number
  • the amine corresponding to Formula 2b comprises at least one allyl group.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2b, the crosslinked polymer is prepared by radical polymerization of an amine corresponding to Formula 2b, and m and z are independently 0, 1, 2 or 3, and n is 0 or 1.
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2b, the crosslinked polymer is prepared by radical polymerization of an amine corresponding to Formula 1, and (i) R 12 or R 42 independently comprise at least one allyl or vinyl moiety, (ii) m is a positive integer and R 22 comprises at least one allyl or vinyl moiety, and/or (iii) n is a positive integer and R 32 comprises at least one allyl moiety.
  • m and z are independently 0, 1, 2 or 3 and n is 0 or 1.
  • R 12 or R 42 in combination comprise at least two allyl or vinyl moieties.
  • m is a positive integer and R 12 , R 22 and R 42 , in combination comprise at least two allyl or vinyl moieties.
  • n is a positive integer and R 12 , R 32 and R 42 , in combination comprise at least two allyl or vinyl moieties.
  • m is a positive integer
  • n is a positive integer
  • the crosslinked polymer comprises the residue of an amine corresponding to Formula 2b
  • the crosslinked polymer is prepared by radical polymerization of an amine corresponding to Formula 2b
  • each R 12 is independently hydrogen, aminoalkyl, allyl, or vinyl
  • R 22 and R 32 are independently hydrogen, alkyl, aminoalkyl, haloalkyl, alkenyl, alkanol, heteroaryl, alicyclic heterocyclic, or aryl
  • R 42 is hydrogen or substituted hydrocarbyl.
  • each R 12 is aminoalkyl, allyl or vinyl
  • R 22 and R 32 are independently hydrogen, alkyl, aminoalkyl, haloalkyl, alkenyl, or alkanol
  • R 42 is hydrogen or substituted hydrocarbyl.
  • each R 12 and R 42 is independently hydrogen, alkyl, allyl, vinyl, —(CH 2 ) d NH 2 or —(CH 2 ) d N[(CH 2 ) e NH 2 ] 2 where d and e are independently 2-4, and R 22 and R 32 are independently hydrogen or heteroaliphatic.
  • Exemplary amines and crosslinkers (or the salts thereof, for example the hydrochloric acid, phosphoric acid, sulfuric acid, or hydrobromic acid salts thereof) for the synthesis of polymers described by Formula 2b include but are not limited to the ones in Table C.
  • the crosslinked polymer is derived from a reaction of the resulting polymers that utilize monomers described in any of Formulae 1, 1a, 1 b, 1c, 2, 2a and 2b or a linear polymer comprised of a repeat unit described by Formula 3 with external crosslinkers or pre-existing polymer functionality that can serve as crosslinking sites.
  • Formula 3 can be a repeat unit of a copolymer or terpolymer where X 15 is either a random, alternating, or block copolymer.
  • the repeating unit in Formula 3 can also represent the repeating unit of a polymer that is branched, or hyperbranched, wherein the primary branch point can be from any atom in the main chain of the polymer
  • R 15 , R 16 and R 17 are independently hydrogen, hydrocarbyl, substituted hydrocarbyl, hydroxyl, amino, boronic acid or halo;
  • X 5 is hydrocarbyl, substituted hydrocarbyl, oxo (—O—), or amino and
  • z is a non-negative number.
  • R 15 , R 16 and R 17 are independently hydrogen, aryl, or heteroaryl, X 5 is hydrocarbyl, substituted hydrocarbyl, oxo or amino, and m and z are non-negative integers. In another embodiment, R 15 , R 16 and R 17 are independently aliphatic or heteroaliphatic, X 5 is hydrocarbyl, substituted hydrocarbyl, oxo (—O—) or amino, and m and z are non-negative integers.
  • R 15 , R 16 and R 17 are independently unsaturated aliphatic or unsaturated heteroaliphatic, X 5 is hydrocarbyl, substituted hydrocarbyl, oxo, or amino, and z is a non-negative integer. In another embodiment, R 15 , R 16 and R 17 are independently alkyl or heteroalkyl, X 5 is hydrocarbyl, substituted hydrocarbyl, oxo, or amino, and z is a non-negative integer.
  • R 15 , R 16 and R 17 are independently alkylamino, aminoalkyl, hydroxyl, amino, boronic acid, halo, haloalkyl, alkanol, or ethereal, X 5 is hydrocarbyl, substituted hydrocarbyl, oxo, or amino, and z is a non-negative integer.
  • R 15 , R 16 and R 17 are independently hydrogen, hydrocarbyl, substituted hydrocarbyl, hydroxyl, amino, boronic acid or halo, X 5 is oxo, amino, alkylamino, ethereal, alkanol, or haloalkyl, and z is a non-negative integer.
  • crosslinking agents that may be used in radical polymerization reactions include, but are not limited to, one or more multifunctional crosslinking agents such as: 1,4-bis(allylamino)butane, 1,2-bis(allylamino)ethane, 2-(allylamino)-1-[2-(allylamino)ethylamino]ethane, 1,3-bis(allylamino)propane, 1,3-bis(allylamino)-2-propanol, triallylamine, diallylamine, divinylbenzene, 1,7-octadiene, 1,6-heptadiene, 1,8-nonadiene, 1,9-decadiene, 1,4-divinyloxybutane, 1,6-hexamethylenebisacrylamide, ethylene bisacrylamide, N,N′-bis(vinylsulfonylacetyl)ethylene diamine, 1,3-bis(vinylsulfonyl) 2-propanol, vinylsulfone,
  • Crosslinked polymers derived from the monomers and polymers in formulas 1 through 3 may be synthesized either in solution or bulk or in dispersed media.
  • solvents that are suitable for the synthesis of polymers of the present disclosure include, but are not limited to water, low boiling alcohols (methanol, ethanol, propanol, butanol), dimethylformamide, dimethylsulfoxide, heptane, chlorobenzene, toluene.
  • Alternative polymer processes may include, a lone polymerization reaction, stepwise addition of individual starting material monomers via a series of reactions, the stepwise addition of blocks of monomers, combinations or any other method of polymerization such as living polymerization, direct polymerization, indirect polymerization, condensation, radical, emulsion, precipitation approaches, spray dry polymerization or using some bulk crosslinking reaction methods and size reduction processes such as grinding, compressing, extrusion.
  • Processes can be carried out as a batch, semi-continuous and continuous processes.
  • the continuous phase can be non-polar solvents, such as toluene, benzene, hydrocarbon, halogenated solvents, super critical carbon dioxide.
  • water can be used and salt can be used to tune the properties of the suspension.
  • the starting molecules described in formulas 1 through 3 may be copolymerized with one or more other monomers of the invention, oligomers or other polymerizable groups.
  • Such copolymer architectures can include, but are not limited to, block or block-like polymers, graft copolymers, and random copolymers.
  • Incorporation of monomers described by formulas 1 through 3 can range from 1% to 99%. In some embodiments, the incorporation of comonomer is between 20% and 80%.
  • Non-limiting examples of comonomers which may be used alone or in combination include: styrene, allylamine hydrochloride, substituted allylamine hydrochloride, substituted styrene, alkyl acrylate, substituted alkyl acrylate, alkyl methacrylate, substituted alkyl methacrylate, acrylonitrile, methacrylonitrile, acrylamide, methacrylamide, N-alkylacrylamide, N-alkylmethacrylamide, N,N-dialkylacrylamide, N,N-dialkylmethacrylamide, isoprene, butadiene, ethylene, vinyl acetate, N-vinyl amide, maleic acid derivatives, vinyl ether, allyle, methallyl monomers and combinations thereof.
  • Additional specific monomers or comonomers that may be used in this invention include, but are not limited to, 2-propen-1-ylamine, 1-(allylamino)-2-aminoethane, 1-[N-allyl(2-aminoethyl)amino]-2-aminoethane, methyl methacrylate, ethyl methacrylate, propyl methacrylate (all isomers), butyl methacrylate (all isomers), 2-ethylhexyl methacrylate, isobornyl methacrylate, methacrylic acid, benzyl methacrylate, phenyl methacrylate, methacrylonitrile, amethylstyrene, methyl acrylate, ethyl acrylate, propyl acrylate (all isomers), butyl acrylate (all isomers), 2-ethylhexyl acrylate, isobornyl
  • Additional modification to the preformed crosslinked polymer can be achieved through the addition of modifiers, including but not limited to amine monomers, additional crosslinkers, and polymers. Modification can be accomplished through covalent or non-covalent methods. These modifications can be evenly or unevenly dispersed throughout the preformed polymer material, including modifications biased to the surface of the preformed crosslinked polymer. Furthermore, modifications can be made to change the physical properties of the preformed crosslinked polymer, including but not limited to reactions that occur with remaining reactive groups such as haloalkyl groups and allyl groups in the preformed polymer. Reactions and modifications to the preformed crosslinked polymer can include but are not limited to acid-base reactions, nucleophilic substitution reactions, Michael reactions, non-covalent electrostatic interactions, hydrophobic interactions, physical interactions (crosslinking) and radical reactions.
  • the post-polymerization crosslinked amine polymer is a crosslinked amine polymer comprising a structure corresponding to Formula 4:
  • each R is independently hydrogen or an ethylene crosslink between two nitrogen atoms of the crosslinked amine polymer
  • a ratio of the sum of a and b to c is in the range of about 1:1 to 5:1.
  • a ratio of the sum of a and b to c i.e., a+b:c
  • a ratio of the sum of a and b to c is in the range of about 1.5:1 to 4:1.
  • a ratio of the sum of a and b to c is in the range of about 1.75:1 to 3:1.
  • a ratio of the sum of a and b is 57, c is 24 and m is large integer indicating an extended polymer network.
  • a ratio of the sum of a and b to c i.e., a+b:c
  • the ratio of the sum of a and b to c i.e., a+b:c
  • the ratio of the sum of a and b to c may be in the range of about 2.2:1 to 2.3:1.
  • the ratio of the sum of a and b to c i.e., a+b:c
  • the ratio of the sum of a and b to c may be in the range of about 2.3:1 to 2.4:1.
  • the ratio of the sum of a and b to c i.e., a+b:c
  • each R may independently be hydrogen or an ethylene crosslink between two nitrogen atoms. Typically, however, 35-95% of the R substituents will be hydrogen and 5-65% will be an ethylene crosslink
  • R substituents will be hydrogen and 5-50% will be an ethylene crosslink
  • R substituents are hydrogen and 10-45% are an ethylene crosslink
  • R substituents are hydrogen and 10-40% are an ethylene crosslink.
  • 65-90% of the R substituents are hydrogen and 10-35% are an ethylene crosslink.
  • a, b, c and R are such that the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 2:1 to about 6:1, respectively.
  • the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 2.5:1 to about 5:1, respectively.
  • the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 3:1 to about 4.5:1, respectively.
  • the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 3.25:1 to about 4.25:1, respectively.
  • the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 3.4:1 to about 4:1, respectively.
  • the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 3.5:1 to about 3.9:1, respectively.
  • the carbon to nitrogen ratio of the polymer of Formula 4 may range from about 3.55:1 to about 3.85:1, respectively.
  • the polymer of Formula 4 is derived from monomers and crosslinkers, each of which comprise less than 5 wt % oxygen.
  • polymers in which crosslinking and/or entanglement were increased were found to have lower swelling than those with lower crosslinking and/or entanglement, yet also had a binding capacity for target ion (e.g., chloride) that was as great as or greater than the lower crosslinking and/or entanglement polymers while binding of interfering ions such as phosphate were significantly reduced.
  • target ion e.g., chloride
  • the selectivity effect may be introduced in two different manners: 1) Overall capacity was sacrificed for chloride specificity. Crosslinkers that don't include chloride binding sites (e.g., epichlorohydrin) allow for increased crosslinking while overall capacity is decreased proportional to the amount of crosslinker incorporated into the polymer. 2) Overall capacity is preserved for chloride specificity: Crosslinkers that include chloride binding sites (e.g., diallylamines) allow for increased crosslinking while overall capacity is staying the same or is reduced by only a small amount.
  • chloride binding sites e.
  • crosslinked polymers having a high capacity for chloride binding and high selectivity for chloride over other competing anions such as phosphate may be prepared in a two-step process in accordance with one embodiment of the present disclosure.
  • the selectivity of the polymer is a function of its crosslinking density and the capacity of the polymer is a function of the free amine density of the crosslinked polymer.
  • the two-step process disclosed herein provides both, high capacity for chloride binding, and high selectivity for chloride over other competing ions by relying primarily upon carbon-carbon crosslinking in the first step, and nitrogen-nitrogen crosslinking in the second step.
  • the crosslinking is preferably capacity-sparing, i.e., free amine sparing, crosslinking from carbon to carbon.
  • the crosslinking is amine-consuming and is directed towards tuning for selectivity.
  • the C—N ratio is preferably optimized to maximize amine functionalities for HCl binding, while still maintaining a spherical polymer particle of controlled particle size to ensure nonabsorption and acceptable mouth feel that is stable under GI conditions.
  • the preferred extent of carbon-carbon crosslinking achieved after the first step is sufficient to permit the resulting bead to swell between 4 ⁇ and 6 ⁇ in water (i.e., a Swelling Ratio of 4 to 6).
  • crosslinked polymers having a high capacity for chloride binding and high selectivity for chloride over other competing anions such as phosphate may be prepared in a two-step process, and the product of the first polymerization step is preferably in the form of beads whose diameter is controlled in the 5 to 1000 micromer range, preferably 10 to 500 micrometers and most preferred 40-180 micrometers.
  • the product of the first polymerization step is preferably in the form of beads whose Swelling Ratio in water is between 2 and 10, more preferably about 3 to about 8, and most preferably about 4 to about 6.
  • the preformed amine polymer is at least partially deprotonated by treatment with a base, preferably a strong base such as a hydroxide base.
  • a base preferably a strong base such as a hydroxide base.
  • the base may be NaOH, KOH, NH 4 OH, NaHCO 3 , Na 2 CO 3 , K 2 CO 3 , LiOH, Li 2 CO 3 , CsOH or other metal hydroxides.
  • the bead will tend to collapse and the crosslinking agent used in the second step may not be able to access binding sites on the polymer unless the bead is prevented from collapsing.
  • One means of preventing the crosslinked polymer bead from collapsing is the use of a swelling agent such as water to swell the bead, thereby allowing the second-step crosslinker to access binding sites.
  • the preformed polymer may be crosslinked to form the post-polymerization crosslinked polymer using any of a range of crosslinking compounds containing at least two amine-reactive functional groups.
  • the crosslinker is a compound containing at least two amine-reactive groups selected from the group consisting of halides, epoxides, phosgene, anhydrides, carbamates, carbonates, isocyanates, thioisocyanates, esters, activated esters, carboxylic acids and derivatives thereof, sulfonates and derivatives thereof, acyl halides, aziridines, ⁇ , ⁇ -unsaturated carbonyls, ketones, aldehydes, and pentafluoroaryl groups.
  • the crosslinker may be, for example, any of the crosslinkers disclosed herein, including a crosslinker selected from Table B.
  • the crosslinker is a dihalide such as a dichloroalkane.
  • a swelling agent for the preformed amine polymer may be included in the reaction mixture for the second polymerization step along with the crosslinking agent.
  • the swelling agent and the crosslinking agent may be miscible or immiscible and the swelling agent may be any composition or combination of compositions that have the capacity to swell the preformed amine polymer.
  • Exemplary swelling agents include polar solvents such as water, methanol, ethanol, n-propanol, isopropanol, n-butanol, formic acid, acetic acid, acetonitrile, dimethylformamide, dimethylsulfoxide, nitromethane, propylene carbonate, or a combination thereof.
  • the amount of swelling agent included in the reaction mixture will typically be less than absorption capacity of the preformed amine polymer for the swelling agent.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture be less than 4:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will be less than 3:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will be less than 2:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will be less than 1:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will be less than 0.5:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will be less than 0.4:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will be less than 0.3:1.
  • the weight ratio of swelling agent to preformed polymer in the reaction mixture will typically be at least 0.05:1, respectively.
  • the crosslinked polymers may be crosslinked homopolymers or crosslinked copolymers comprising free amine moieties.
  • the free amine moieties may be separated, for example, by the same or varying lengths of repeating linker (or intervening) units.
  • the polymers comprise repeat units containing an amine moiety and an intervening linker unit.
  • multiple amine-containing repeat units are separated by one or more linker units.
  • the polyfunctional crosslinkers may comprise HCl binding functional groups, e.g., amines, (“active crosslinkers”) or may lack HCl binding functional groups such as amines (“passive crosslinkers”).
  • the first polymerization (crosslinking) step yields preformed amine polymer beads having a target size and chloride binding capacity.
  • the beads have a chloride binding capacity of at least 10 mmol/g in Simulated Gastric Fluid (“SGF”) and a Swelling Ratio in the range of 1 to 6.
  • SGF Simulated Gastric Fluid
  • the resulting preformed amine polymer is then preferably (at least partially) deprotonated with a base and combined with a non-protonating swelling agent to swell the free amine polymer without protonating the amine functions.
  • the amount of the non-protonating swelling agent is selected to tune the subsequent degree of crosslinking effectively forming a template that is then locked into place via the amine consuming crosslinking step.
  • the second crosslinking step the swollen, deprotonated preformed amine polymer is crosslinked with a crosslinker containing amine reactive moieties to form a post-polymerization crosslinked polymer.
  • selectivity for chloride over other competing ions is achieved with highly crosslinked polymers.
  • relatively high chloride binding capacity maybe be attained by reacting a preformed amine polymer bead with neat crosslinker in the presence of a swelling agent (water). While this “non-dispersed” reaction provides access to high selectivity for chloride over competing ions in the SIB assay, it also results in macroscopically (and microscopically) aggregated polymer beads.
  • a solvent e.g., heptane
  • DCE was discovered to have excellent dispersal properties as a solvent, when compared to similar reactions with DCP and/or heptane. Additionally, less aggregation was observed when the beads were first dispersed in DCE and then in a second operation, the water is added to swell the beads. If water is added to the preformed amine polymer before the bead is dispersed in the DCE, aggregation may occur.
  • DCE 1,2-dichloroethane
  • the reaction mixture may contain a wide range of amounts of crosslinking agents.
  • the crosslinker may be used in large excess relative to the amount of preformed amine polymer in the reaction mixtures.
  • the crosslinking agent is a crosslinking solvent, i.e., it is both a solvent for the reaction mixture and a crosslinking agent for the preformed amine polymer.
  • other solvents may optionally be included in the reaction mixture but are not required.
  • the preformed amine polymer, swelling agent and crosslinker may be dispersed in a solvent that is miscible with the crosslinker and immiscible with the swelling agent.
  • the swelling agent may be a polar solvent; in some such embodiments, for example, the swelling agent may comprise water, methanol, ethanol, n-propanol, isopropanol, formic acid, acetic acid, acetonitrile, N,N-dimethylformamide, dimethylsulfoxide, nitromethane, or a combination thereof.
  • the solvent system for the reaction mixture will typically comprise a non-polar solvent such as pentane, cyclopentane, hexane, cyclohexane, benzene, toluene, 1,4-dioxane, chloroform, diethyl ether, dichloromethane, dichloroethane, dichloropropane, dichlorobutane, or a combination thereof.
  • a non-polar solvent such as pentane, cyclopentane, hexane, cyclohexane, benzene, toluene, 1,4-dioxane, chloroform, diethyl ether, dichloromethane, dichloroethane, dichloropropane, dichlorobutane, or a combination thereof.
  • the crosslinker and the solvent may be the same; i.e., the solvent is a crosslinking solvent such as 1,2-dichloroethane, 1,3-dichloropropane, 1,4-dichlorobutane or a combination thereof.
  • the solvent is a crosslinking solvent such as 1,2-dichloroethane, 1,3-dichloropropane, 1,4-dichlorobutane or a combination thereof.
  • crosslinking solvent e.g., a DCE-dispersed reaction
  • there is a large excess of crosslinker regardless of the amount of crosslinking solvent (e.g., DCE) used to disperse the bead (e.g., both 1 g:3 mL::bead:DCE and 1 g:10 mL::bead:DCE are a large excess of crosslinker, most of which is not consumed during the reaction).
  • the relative degree of crosslinking, and the performance in SIB assay are unaffected by changes in the ratio of reactive crosslinker to polymer bead. This is possible because the reaction is limited by the acid-neutralizing capacity of the polymer bead, rather than the amount of crosslinker (e.g., DCE).
  • the amines of the preformed polymer bead preferably have a free electron pair (neutral, deprotonated).
  • the crosslinker e.g., DCE
  • HCl is produced and the amines become protonated, thus limiting the reaction.
  • the preformed amine polymer beads preferably start as the free amine in the second crosslinking step. If the preformed amine polymer bead is protonated after the first step of carbon-carbon crosslinking, amine-consuming crosslinking in the second step will be limited, thus reducing the desired selectivity for chloride over other competing ions.
  • the benefits of deprotonated preformed polymer beads in the second step crosslinking highlights the advantages of using two steps to achieve the final product.
  • the first step to form the amine polymer bead, all monomers (e.g., allylamine and DAPDA) are protonated to remain in the aqueous phase and to avoid the radical transfer reactions that severely limit the polymerization of non-protonated allylamine (and derivatives).
  • the bead can then be deprotonated and further crosslinked with an amine reactive crosslinker in a second step.
  • the first reaction step comprises radical polymerization.
  • the amine monomer will typically be a mono-functional vinyl, allyl, or acrylamide (e.g., allylamine) and crosslinkers will have two or more vinyl, allyl or acrylamide functionalities (e.g., diallylamine).
  • Concurrent polymerization and crosslinking occurs through radically initiated polymerization of a mixture of the mono- and multifunctional allylamines. The resulting polymer network is thusly crosslinked through the carbon backbone.
  • Each crosslinking reaction forms a carbon-carbon bond (as opposed to substitution reactions in which a carbon-heteroatom bond is formed during crosslinking).
  • the amine functionalities of the monomers do not undergo crosslinking reactions and are preserved in the final polymer (i.e., primary amines remain primary, secondary amines remain secondary, and tertiary amines remain tertiary).
  • a wide range of initiators may be used including cationic and radical initiators.
  • suitable initiators include: the free radical peroxy and azo type compounds, such as azodiisobutyronitrile, azodiisovaleronitrile, dimethylazodiisobutyrate, 2,2′azo bis(isobutyronitrile), 2,2′-azobis(N,N′-dimethyl-eneisobutyram idine)dihydrochloride, 2,2′-azobis(2-amidinopropane)dihydrochloride, 2,2′-azobis(N,N′-dimethyleneisobutyramidine), 1,1′-azo bis(I-cyclohexanecarbo-nitrile), 4,4′-azobis(4-cyanopentanoic acid), 2,2′-azobis(isobutyramide)dihydrate, 2,2′-azobis(2-methylpropane
  • azo type compounds such as azodiisobutyronitrile,
  • Exemplary amine-containing polymers as described above are more fully disclosed and exemplified in WO2016/094685 A1 and WO2014/197725 A1, the entire contents of which are incorporated herein by reference.
  • the pharmaceutical composition comprises a mixture of any of the previously-identified nonabsorbable materials.
  • the pharmaceutical composition comprises a mixture of a cation exchange composition with at least one anion exchange composition, amphoteric ion exchange composition, or neutral composition having the capacity to bind both protons and anions.
  • the pharmaceutical composition comprises a mixture of an anion exchange composition with at least one cation exchange composition, amphoteric ion exchange composition, or neutral composition having the capacity to bind both protons and anions.
  • the pharmaceutical composition comprises a mixture of a neutral composition having the capacity to bind both protons and anions with at least one cation exchange composition, amphoteric ion exchange composition, or anion exchange composition.
  • a nonabsorbable free-amine polymer of the present disclosure is orally ingested and used to treat metabolic acidosis (including by increasing serum bicarbonate and normalizing blood pH) in a mammal by binding HCl in the gastrointestinal (“GI”) tract and removing HCl through the feces.
  • Free-amine polymer is taken orally ( FIG. 1A ) at compliance enhancing dose targeted to chronically bind sufficient amounts of HCl to enable clinically meaningful increase in serum bicarbonate of 3 mEq/L.
  • free amine becomes protonated by binding H + .
  • Positive charge on polymer is then available to bind Cl ⁇ ; by controlling access of binding sites through crosslinking and hydrophilicity/hydrophobicity properties, other larger organic anions (e.g., acetate, propionate, butyrate, etc., depicted as X ⁇ and Y ⁇ ) are bound to a lesser degree, if at all. The net effect is therefore binding of HCl.
  • Cl ⁇ is not fully released and HCl is removed from the body through regular bowel movement and fecal excretion, resulting in net alkalinization in the serum. Cl ⁇ bound in this fashion is not available for exchange via the Cl ⁇ /HCO 3 ⁇ antiporter system.
  • the polymer is designed to simultaneously maximize efficacy (net HCl binding and excretion) and minimize GI side effects (through low swelling particle design and particle size distribution).
  • Optimized HCl binding may be accomplished through a careful balance of capacity (number of amine binding sites), selectivity (preferred binding of chloride versus other anions, in particular organic anions in the colon) and retention (not releasing significant amounts of chloride in the lower GI tract to avoid the activity of the Cl ⁇ /HCO 3 ⁇ exchanger [antiporter] in the colon and intestine; if chloride is not tightly bound to the polymer the Cl ⁇ /HCO 3 ⁇ exchanger can mediate uptake of chloride ion from the intestinal lumen and reciprocal exchange for bicarbonate from the serum, thus effectively decreasing serum bicarbonate.
  • Competing anions that displace chloride lead to a decrease in net bicarbonate through the following mechanisms.
  • displacement of chloride from the polymer in the GI lumen, particularly the colon lumen provides for a facile exchange with bicarbonate in the serum.
  • the colon has an anion exchanger (chloride/bicarbonate antiporter) that moves chloride from the luminal side in exchange for secreted bicarbonate.
  • chloride/bicarbonate antiporter chloride/bicarbonate antiporter
  • Short chain fatty acids are the product of bacterial metabolism of complex carbohydrates that are not catabolized by normal digestive processes (Chemlarova, 2007). Short chain fatty acids that reach the colon are absorbed and distributed to various tissues, with the common metabolic fate being the generation of H 2 O and CO 2 , which is converted to bicarbonate equivalents.
  • binding of SCFA to the polymer to neutralize the proton charge would be detrimental to overall bicarbonate stores and buffering capacity, necessitating the design of chemical and physical features in the polymer that limit SCFA exchange.
  • phosphate binding to the polymer should be limited as well, since phosphate represents an additional source of buffering capacity in the situation where ammoniagenesis and/or hydrogen ion secretion is compromised in chronic renal disease.
  • an anion is preferably bound as the positive charge seeks to leave the human body as a neutral polymer.
  • Binding is more than minimal binding, i.e., at least about 0.2 mmol of ion/g of polymer, at least about 1 mmol of ion/g of polymer in some embodiments, at least about 1.5 mmol of ion/g of polymer in some embodiments, at least about 3 mmol of ion/g of polymer in some embodiments, at least about 5 mmol of ion/g of polymer in some embodiments, at least about 10 mmol of ion/g of polymer in some embodiments, at least about 12 mmol of ion/g of polymer in some embodiments, at least about 13 mmol of ion/g of polymer in some embodiments, or even at least about 14 mmol of ion/g of polymer in some embodiments.
  • the polymers are characterized by their high capacity of proton binding while at the same time providing selectivity for anions; selectivity for chloride is accomplished by reducing the binding of interfering anions that include but are not limited to phosphate, citrate, acetate, bile acids and fatty acids.
  • selectivity for chloride is accomplished by reducing the binding of interfering anions that include but are not limited to phosphate, citrate, acetate, bile acids and fatty acids.
  • polymers of the present disclosure bind phosphate with a binding capacity of less than about 5 mmol/g, less than about 4 mmol/g, less than about 3 mmol/g, less than about 2 mmol/g or even less than about 1 mmol/g.
  • polymers of the invention bind bile and fatty acids with a binding capacity of less than about less than about 5 mmol/g, less than about 4 mmol/g, less than about 3 mmol/g, less than about 2 mmol/g, less than about 1 mmol/g in some embodiments, less than about 0.5 mmol/g in some embodiments, less than about 0.3 mmol/g in some embodiments, and less than about 0.1 mmol/g in some embodiments.
  • the dosage levels of the nonabsorbable compositions for therapeutic and/or prophylactic uses may range from about 0.5 g/day to about 100 g/day.
  • the dose be in the range of about 1 g/day to about 50 g/day.
  • the dose will be about 2 g/day to about 25 g/day.
  • the dose will be about 3 g/day to about 25 g/day.
  • the dose will be about 4 g/day to about 25 g/day.
  • the dose will be about 5 g/day to about 25 g/day.
  • the dose will be about 2.5 g/day to about 20 g/day.
  • the dose will be about 2.5 g/day to about 15 g/day.
  • the dose will be about 1 g/day to about 10 g/day.
  • the daily dose may be administered as a single dose (i.e., one time a day), or divided into multiple doses (e.g., two, three or more doses) over the course of a day.
  • the nonabsorbable compositions may be administered as a fixed daily dose or titrated based on the serum bicarbonate values of the patient in need of treatment or other indicators of acidosis. The titration may occur at the onset of treatment or throughout, as required, and starting and maintenance dosage levels may differ from patient to patient based on severity of the underlying disease.
  • the effectiveness of the nonabsorbable composition may be established in animal models, or in human volunteers and patients.
  • in vitro, ex vivo and in vivo approaches are useful to establish HCl binding.
  • In vitro binding solutions can be used to measure the binding capacity for proton, chloride and other ions at different pHs.
  • Ex vivo extracts such as the gastrointestinal lumen contents from human volunteers or from model animals can be used for similar purposes. The selectivity of binding and/or retaining certain ions preferentially over others can also be demonstrated in such in vitro and ex vivo solutions.
  • the nonabsorbable compositions are provided (by oral administration) to an animal, including a human, in a dosing regimen of one, two or even multiple (i.e., at least three) doses per day to treat an acid-base disorder (e.g., metabolic acidosis) and achieve a clinically significant and sustained increase of serum bicarbonate as previously described.
  • an acid-base disorder e.g., metabolic acidosis
  • a daily dose of the nonabsorbable composition (whether orally administered in a single dose or multiple doses over the course of the day) has sufficient capacity to remove at least 5 mmol of protons, chloride ions or each per day.
  • a daily dose of the nonabsorbable composition has sufficient capacity to remove at least 10 mmol of protons, chloride ions or each per day.
  • a daily dose of the nonabsorbable composition has sufficient capacity to remove at least 20 mmol of protons, the conjugate base of a strong acid (e.g., Cl ⁇ , HSO 4 ⁇ and SO 4 2 ⁇ ) and/or a strong acid (e.g., HCl or H 2 SO 4 ) each per day.
  • a strong acid e.g., Cl ⁇ , HSO 4 ⁇ and SO 4 2 ⁇
  • a strong acid e.g., HCl or H 2 SO 4
  • a daily dose of the nonabsorbable composition has sufficient capacity to remove at least 30 mmol of protons, the conjugate base of a strong acid, and/or a strong acid each per day.
  • a daily dose of the nonabsorbable composition has sufficient capacity to remove at least 40 mmol of protons, the conjugate base of a strong acid, and/or a strong acid each per day.
  • a daily dose of the nonabsorbable composition has sufficient capacity to remove at least 50 mmol of protons, the conjugate base of a strong acid, and/or a strong acid each per day.
  • the dosage unit form of the pharmaceutical comprising the nonabsorbable composition may be any form appropriate for oral administration. Such dosage unit forms include powders, tablets, pills, lozenges, sachets, cachets, elixirs, suspensions, syrups, soft or hard gelatin capsules, and the like.
  • the pharmaceutical composition comprises only the nonabsorbable composition.
  • the pharmaceutical composition may comprise a carrier, a diluent, or excipient in addition to the nonabsorbable composition.
  • Examples of carriers, excipients, and diluents that may be used in these formulations as well as others, include foods, drinks, lactose, dextrose, sucrose, sorbitol, mannitol, starches, gum acacia, alginates, tragacanth, gelatin, calcium silicate, microcrystalline cellulose, polyvinylpyrrolidone, cellulose, methyl cellulose, methylhydroxybenzoates, propylhydroxybenzoates, propylhydroxybenzoates, and talc.
  • compositions further include a binder, such as microcrystalline cellulose, colloidal silica and combinations thereof (Prosolv 90), carbopol, providone and xanthan gum; a flavoring agent, such as sucrose, mannitol, xylitol, maltodextrin, fructose, or sorbitol; a lubricant, such as magnesium stearate, stearic acid, sodium stearyl fumurate and vegetable based fatty acids; and, optionally, a disintegrant, such as croscarmellose sodium, gellan gum, low-substituted hydroxypropyl ether of cellulose, sodium starch glycolate.
  • a binder such as microcrystalline cellulose, colloidal silica and combinations thereof (Prosolv 90), carbopol, providone and xanthan gum
  • a flavoring agent such as sucrose, mannitol, xylitol, maltodextrin, fructose, or sorbitol
  • additives may include plasticizers, pigments, talc, and the like.
  • plasticizers pigments, talc, and the like.
  • suitable ingredients are well-known in the art; see, e.g., Gennaro A R (ed), Remington's Pharmaceutical Sciences, 20th Edition.
  • the nonabsorbable composition may be co-administered with other active pharmaceutical agents depending on the condition being treated.
  • This co-administration may include simultaneous administration of the two agents in the same dosage form, simultaneous administration in separate dosage forms, and separate administration.
  • the nonabsorbable composition may be co-administered with common treatments that are required to treat underlying co-morbidities including but not limited to edema, hypertension, diabetes, obesity, heart failure and complications of Chronic Kidney Disease.
  • These medications and the nonabsorbable composition can be formulated together in the same dosage form and administered simultaneously as long as they do not display any clinically significant drug-drug-interactions.
  • these treatments and the nonabsorbable composition may be separately and sequentially administered with the administration of one being followed by the administration of the other.
  • the daily dose of the chronic metabolic acidosis treatment is compliance enhancing (approximately 15 g or less per day) and achieves a clinically significant and sustained increase of serum bicarbonate of approximately 3 mEq/L at these daily doses.
  • the non-absorbed nature of the polymer and the lack of sodium load and/or introduction of other deleterious ions for such an oral drug enable for the first time a safe, chronic treatment of metabolic acidosis without worsening blood pressure/hypertension and/or without causing increased fluid retention and fluid overload.
  • Another benefit is further slowing of the progression of kidney disease and time to onset of lifelong renal replacement therapy (End Stage Renal Disease “ESRD” including 3 times a week dialysis) or need for kidney transplants. Both are associated with significant mortality, low quality of life and significant burden to healthcare systems around the world. In the United States alone, approximately 20% of the 400,000 ESRD patients die and 100,000 new patients start dialysis every year.
  • a further aspect of the present disclosure is a pharmaceutical product comprising a sealed package and the nonabsorbable composition of the present disclosure within the sealed package.
  • the sealed package is preferably substantially impermeable to moisture and oxygen to increase the stability of the pharmaceutical composition.
  • the dosage unit form may comprise a sealed container (e.g., a sealed sachet) that prevents or reduces ingress of moisture and oxygen upon packaging the nonabsorbable composition in the container.
  • the container size can be optimized to reduce head space in the container after packaging and any head space may be filled with an inert gas such as nitrogen.
  • container material of construction can be chosen to minimize the moisture and oxygen ingress inside the container after packaging.
  • the nonabsorbable composition may be packaged in a multilayer sachet containing at least one or more layer that serves as a barrier layer to moisture and oxygen ingress.
  • the nonabsorbable composition may be packaged in a single layer or multilayer plastic, metal or glass container that has at least one or more barrier layers incorporated in the structure that limits oxygen and/or moisture ingress after packaging.
  • the sachet (or other container or package) may comprise a multi-layer laminate of an inner contact layer, an outer layer; and a barrier layer disposed between the contact layer and outer layer.
  • the container includes one or more oxygen-scavenging layers.
  • a method of treating an individual afflicted with an acid-base disorder characterized by a baseline serum bicarbonate value of less than 22 mEq/l comprising oral administration of a daily dose of a pharmaceutical composition having the capacity to bind at least 5 mEq of a target species as it transits the digestive system to achieve a clinically significant increase in the serum bicarbonate value of at least 1 mEq/l from baseline within a treatment period not greater than 1 month, the target species being selected from the group consisting of protons, strong acids, and conjugate bases of strong acids.
  • a method of treating an individual afflicted with an acid-base disorder characterized by a baseline serum bicarbonate value of less than 22 mEq/l comprising oral administration of a pharmaceutical composition, wherein the pharmaceutical composition given orally binds at least 5 mEq per day on average of a target species in the digestive system, said oral administration achieving a clinically significant increase in the serum bicarbonate value of at least 1 mEq/l from baseline within a treatment period not greater than 1 month, the target species being selected from the group consisting of protons, strong acids, and conjugate bases of strong acids.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least 22 mEq/l.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least 23 mEq/l.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least 24 mEq/l.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least mEq/l.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least 26 mEq/l.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least 27 mEq/l.
  • any preceding enumerated embodiment wherein the method increases the serum bicarbonate value from the baseline serum bicarbonate value to an increased serum bicarbonate value of at least 28 mEq/l.
  • the baseline serum bicarbonate value is the value of the serum bicarbonate concentration determined at a single time point.
  • baseline serum bicarbonate value is the mean value of at least two serum bicarbonate concentrations determined at different time-points.
  • baseline serum bicarbonate value is the mean value of at least two serum bicarbonate concentrations for serum samples drawn on different days.
  • the method of embodiment 249 wherein the baseline serum bicarbonate value is the mean value of at least two serum bicarbonate concentrations for serum samples drawn on consecutive days.
  • the baseline serum bicarbonate value is the mean value of at least two serum bicarbonate concentrations for serum samples drawn on two consecutive days and prior to the initiation of the treatment.
  • the baseline serum bicarbonate value is the mean or median value of at least two serum bicarbonate concentrations for serum samples drawn on non-consecutive days.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 7.5 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 10 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 15 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 20 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 25 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 30 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 35 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 40 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 45 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 50 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 55 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 60 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 65 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 70 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 75 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 80 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 85 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 90 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 95 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 100 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 105 mEq of a target species as it transits the digestive system.
  • any preceding enumerated embodiment wherein the daily dose has the capacity to remove at least 110 mEq of a target species as it transits the digestive system.
  • composition is a nonabsorbable composition 15 comprising a population of particles having a median particle diameter size (volume distribution) of at least 3 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 5 to 1,000 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 5 to 500 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 10 to 400 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 10 to 300 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 20 to 250 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 30 to 250 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a median particle diameter size (volume distribution) in the range of 40 to 180 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles in which less than 7% of the particles in the population (volume distribution) have a diameter less than 10 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles in which less than 5% of the particles in the particles in the population (volume distribution) have a diameter less than 10 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles in which less than 2.5% of the particles in the particles in the population (volume distribution) have a diameter less than 10 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles in which less than 1% of the particles in the particles in the population (volume distribution) have a diameter less than 10 microns.
  • the pharmaceutical composition is a nonabsorbable composition comprising a population of particles having a particle size range that is (i) large enough to avoid passive or active absorption through the GI tract and (ii) small enough to not cause grittiness or unpleasant mouth feel when ingested as a powder, suspension, gel, and/or tablet.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 9.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 8.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 7.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 6.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 5.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 4.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 3.
  • composition is a nonabsorbable composition comprising a population of particles have a Swelling Ratio of less than 2.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 0.5 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 1 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 2 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 3 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 4 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 5 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 7.5 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 10 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 12.5 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 15 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 20 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 25 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 30 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species of at least about 35 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 2 to 25 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 3 to 25 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 5 to 25 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 10 to 25 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 5 to 20 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 6 to 20 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 7.5 to 20 mEq/g.
  • nonabsorbable composition has a theoretical binding capacity for the target species in the range of 10 to 20 mEq/g.
  • the target species comprises the conjugate base of a strong acid.
  • the target species comprises the conjugate base of a strong acid selected from the group consisting of chloride, bisulfate and sulfate ions.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 1 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 1.5 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion 15 binding capacity of at least 2 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 2.5 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 3 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 3.5 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 4 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 4.5 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 5 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 5.5 mEq/g in a SIB assay.
  • nonabsorbable composition is characterized by a chloride ion binding capacity of at least 6 mEq/g in a SIB assay.

Landscapes

  • Health & Medical Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Medicinal Chemistry (AREA)
  • Pharmacology & Pharmacy (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Animal Behavior & Ethology (AREA)
  • General Health & Medical Sciences (AREA)
  • Public Health (AREA)
  • Veterinary Medicine (AREA)
  • Epidemiology (AREA)
  • Organic Chemistry (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Bioinformatics & Cheminformatics (AREA)
  • Engineering & Computer Science (AREA)
  • General Chemical & Material Sciences (AREA)
  • Nuclear Medicine, Radiotherapy & Molecular Imaging (AREA)
  • Polymers & Plastics (AREA)
  • Physiology (AREA)
  • Nutrition Science (AREA)
  • Hematology (AREA)
  • Obesity (AREA)
  • Diabetes (AREA)
  • Inorganic Chemistry (AREA)
  • Urology & Nephrology (AREA)
  • Dispersion Chemistry (AREA)
  • Pharmaceuticals Containing Other Organic And Inorganic Compounds (AREA)
  • Acyclic And Carbocyclic Compounds In Medicinal Compositions (AREA)
  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
  • Medicinal Preparation (AREA)
  • Addition Polymer Or Copolymer, Post-Treatments, Or Chemical Modifications (AREA)
US16/099,045 2016-05-06 2017-05-05 Compositions for and methods of treating acid-base disorders Abandoned US20200054669A1 (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
US16/099,045 US20200054669A1 (en) 2016-05-06 2017-05-05 Compositions for and methods of treating acid-base disorders

Applications Claiming Priority (6)

Application Number Priority Date Filing Date Title
US201662333059P 2016-05-06 2016-05-06
US201662350686P 2016-06-15 2016-06-15
US201662408885P 2016-10-17 2016-10-17
US201662414966P 2016-10-31 2016-10-31
US16/099,045 US20200054669A1 (en) 2016-05-06 2017-05-05 Compositions for and methods of treating acid-base disorders
PCT/US2017/031395 WO2017193064A1 (en) 2016-05-06 2017-05-05 Compositions for and method of treating acid-base disorders

Related Parent Applications (1)

Application Number Title Priority Date Filing Date
PCT/US2017/031395 A-371-Of-International WO2017193064A1 (en) 2016-05-06 2017-05-05 Compositions for and method of treating acid-base disorders

Related Child Applications (1)

Application Number Title Priority Date Filing Date
US17/485,177 Continuation US11992501B2 (en) 2016-05-06 2021-09-24 Compositions for and methods of treating acid-base disorders

Publications (1)

Publication Number Publication Date
US20200054669A1 true US20200054669A1 (en) 2020-02-20

Family

ID=59315687

Family Applications (6)

Application Number Title Priority Date Filing Date
US16/099,029 Abandoned US20190209607A1 (en) 2016-05-06 2017-05-05 Compositions for treating acid-base disorders
US16/099,045 Abandoned US20200054669A1 (en) 2016-05-06 2017-05-05 Compositions for and methods of treating acid-base disorders
US16/099,024 Active 2039-01-01 US11406661B2 (en) 2016-05-06 2017-05-05 HCl-binding compositions for and methods of treating acid-base disorders
US17/192,701 Pending US20210205351A1 (en) 2016-05-06 2021-03-04 Compositions for treating acid-base disorders
US17/485,177 Active 2037-10-03 US11992501B2 (en) 2016-05-06 2021-09-24 Compositions for and methods of treating acid-base disorders
US17/878,192 Pending US20250009785A1 (en) 2016-05-06 2022-08-01 Hcl-binding compositions for and methods of treating acid-base disorders

Family Applications Before (1)

Application Number Title Priority Date Filing Date
US16/099,029 Abandoned US20190209607A1 (en) 2016-05-06 2017-05-05 Compositions for treating acid-base disorders

Family Applications After (4)

Application Number Title Priority Date Filing Date
US16/099,024 Active 2039-01-01 US11406661B2 (en) 2016-05-06 2017-05-05 HCl-binding compositions for and methods of treating acid-base disorders
US17/192,701 Pending US20210205351A1 (en) 2016-05-06 2021-03-04 Compositions for treating acid-base disorders
US17/485,177 Active 2037-10-03 US11992501B2 (en) 2016-05-06 2021-09-24 Compositions for and methods of treating acid-base disorders
US17/878,192 Pending US20250009785A1 (en) 2016-05-06 2022-08-01 Hcl-binding compositions for and methods of treating acid-base disorders

Country Status (15)

Country Link
US (6) US20190209607A1 (enExample)
EP (3) EP3452028A4 (enExample)
JP (3) JP7071284B2 (enExample)
KR (1) KR102655774B1 (enExample)
CN (2) CN116211887A (enExample)
AU (3) AU2017261337A1 (enExample)
BR (1) BR112018072714A2 (enExample)
CA (1) CA3023264A1 (enExample)
IL (2) IL262660B2 (enExample)
MA (3) MA44886A (enExample)
MX (1) MX2018013476A (enExample)
MY (1) MY197091A (enExample)
RU (1) RU2018142943A (enExample)
SG (1) SG11201809605PA (enExample)
WO (3) WO2017193024A1 (enExample)

Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US11406661B2 (en) 2016-05-06 2022-08-09 Tricida, Inc. HCl-binding compositions for and methods of treating acid-base disorders
US11738041B2 (en) 2014-12-10 2023-08-29 Renosis, Inc. Proton-binding polymers for oral administration
US11986490B2 (en) 2017-11-03 2024-05-21 Renosis, Inc. Compositions for and method of treating acid-base disorders

Families Citing this family (10)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
HRP20171590T1 (hr) 2013-06-05 2017-12-29 Tricida Inc. Polimeri koji vežu protone za oralnu primjenu
US10934380B1 (en) 2017-09-25 2021-03-02 Tricida, Inc. Crosslinked poly(allylamine) polymer pharmaceutical compositions
CA3079171C (en) * 2017-10-16 2023-09-12 Fujifilm Corporation Therapeutic agent for hyperphosphatemia and particles
AU2018360868B2 (en) * 2017-11-03 2025-01-02 Tricida, Inc. Method of treating acid-base disorders
CA3102765A1 (en) * 2018-06-04 2019-12-12 Tricida, Inc. Method of treating acid-base disorders
WO2019236639A1 (en) * 2018-06-04 2019-12-12 Tricida, Inc. Method of treating acid-base disorders
FI4053179T3 (fi) 2021-03-01 2025-11-26 Renosis Inc Silloitettujen poly(allyyliamiini)polymeerien lääkekoostumuksia
CA3212512A1 (en) 2021-03-01 2022-09-09 Renosis, Inc. Crosslinked poly(allylamine) polymer pharmaceutical compositions
CN118510524A (zh) * 2021-12-14 2024-08-16 上海石趣医药科技有限公司 氧化银和/或其水合物在制备药物中的用途
WO2023109826A1 (zh) * 2021-12-14 2023-06-22 上海石趣医药科技有限公司 碳酸银在制备药物中的用途

Citations (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20160074430A1 (en) * 2013-06-05 2016-03-17 Tricida, Inc. Proton-binding polymers for oral administration

Family Cites Families (115)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20050090553A1 (en) 1992-06-30 2005-04-28 Shapiro Howard K. Compositions and method for treatment of chronic inflammatory diseases
US6444221B1 (en) 1992-06-30 2002-09-03 Howard K. Shapiro Methods of treating chronic inflammatory diseases using carbonyl trapping agents
US5667775A (en) 1993-08-11 1997-09-16 Geltex Pharmaceuticals, Inc. Phosphate-binding polymers for oral administration
US5496545A (en) 1993-08-11 1996-03-05 Geltex Pharmaceuticals, Inc. Phosphate-binding polymers for oral administration
US5648355A (en) 1994-02-09 1997-07-15 Kos Pharmaceutical, Inc. Method of treatment of endogenous, painful gastrointestinal conditions of non-inflammatory, non-ulcerative origin
TW474813B (en) 1994-06-10 2002-02-01 Geltex Pharma Inc Alkylated composition for removing bile salts from a patient
AU703842B2 (en) 1994-10-17 1999-04-01 Robert M. Bersin Compositions comprising carbonate/bicarbonate buffered dichloroacetic acid and methods for treatment of metabolic and cardiovascular disorders
US20020006899A1 (en) 1998-10-06 2002-01-17 Pospisilik Andrew J. Use of dipeptidyl peptidase IV effectors for lowering blood pressure in mammals
US5753706A (en) 1996-12-16 1998-05-19 Hsu; Chen Hsing Methods for treating renal failure
AUPO758297A0 (en) 1997-06-27 1997-07-24 Rowe, James Baber Control of acidic gut syndrome
US6726905B1 (en) 1997-11-05 2004-04-27 Genzyme Corporation Poly (diallylamines)-based phosphate binders
WO1999040990A1 (en) 1998-02-17 1999-08-19 University Of Maryland Anion binding polymers and the use thereof
US6485703B1 (en) 1998-07-31 2002-11-26 The Texas A&M University System Compositions and methods for analyte detection
US6271264B1 (en) 1998-12-01 2001-08-07 Geltex Pharmaceuticals, Inc. Polymers containing spirobicyclic ammonium moieties as bile acid sequestrants
US6733780B1 (en) 1999-10-19 2004-05-11 Genzyme Corporation Direct compression polymer tablet core
GB9927088D0 (en) 1999-11-17 2000-01-12 Secr Defence Use of poly(diallylamine) polymers
US6844372B2 (en) 2000-03-09 2005-01-18 Hisamitsu Pharmaceutical Co., Inc. Crosslinked anion-exchange resin or salt thereof and phosphorus adsorbent comprising the same
WO2001066606A1 (en) 2000-03-09 2001-09-13 Hisamitsu Pharmaceutical Co., Inc. Crosslinked anion-exchange resin or salt thereof
WO2001068106A1 (en) 2000-03-13 2001-09-20 Hisamitsu Pharmaceutical Co., Inc. Preventives and/or remedies for hyperphosphatemia
JP2002028737A (ja) 2000-07-07 2002-01-29 Fujitsu Ltd プレス打ち抜き加工方法及びプレス打ち抜き加工装置
AT409630B (de) * 2000-12-13 2002-09-25 Dsm Fine Chem Austria Gmbh Alkylierung von n-bzw. amino- oder ammoniumgruppen haltigen, vernetzten polymeren
BR0209020A (pt) 2001-04-18 2004-08-10 Genzyme Corp Composição farmacêutica de polialilamina
EP1416942B1 (en) 2001-04-18 2007-12-12 Genzyme Corporation Amine polymers for treating gout and binding uric acid
EP1483232A1 (en) 2002-03-11 2004-12-08 Novartis AG Salts of nateglinide
AU2004210013A1 (en) 2003-02-10 2004-08-19 Autogen Research Pty Ltd Therapeutic molecules
TWI335218B (en) 2003-02-19 2011-01-01 Panion & Bf Biotech Inc Ferric organic compounds, uses thereof and methods of making same
US7335795B2 (en) 2004-03-22 2008-02-26 Ilypsa, Inc. Crosslinked amine polymers
US7767768B2 (en) 2003-11-03 2010-08-03 Ilypsa, Inc. Crosslinked amine polymers
US7385012B2 (en) 2003-11-03 2008-06-10 Ilypsa, Inc. Polyamine polymers
US7449605B2 (en) 2003-11-03 2008-11-11 Ilypsa, Inc. Crosslinked amine polymers
US7608674B2 (en) 2003-11-03 2009-10-27 Ilypsa, Inc. Pharmaceutical compositions comprising cross-linked small molecule amine polymers
US7459502B2 (en) 2003-11-03 2008-12-02 Ilypsa, Inc. Pharmaceutical compositions comprising crosslinked polyamine polymers
CA2551528A1 (en) 2003-12-31 2005-07-21 Genzyme Corporation Enteric coated aliphatic amine polymer bile acid sequestrants
CA2553931A1 (en) 2004-01-29 2005-08-11 Keio University Erythrocyte function modifying substance
US8192758B2 (en) 2004-03-30 2012-06-05 Relypsa, Inc. Ion binding compositions
US7854924B2 (en) 2004-03-30 2010-12-21 Relypsa, Inc. Methods and compositions for treatment of ion imbalances
US8282960B2 (en) 2004-03-30 2012-10-09 Relypsa, Inc. Ion binding compositions
US7556799B2 (en) 2004-03-30 2009-07-07 Relypsa, Inc. Ion binding polymers and uses thereof
US7429394B2 (en) 2004-03-30 2008-09-30 Relypsa, Inc. Ion binding compositions
PL1732523T3 (pl) 2004-03-30 2010-08-31 Vifor Pharma Tech Ltd Polimery wiążące potas i ich zastosowania
US8399025B2 (en) 2004-06-04 2013-03-19 Board Of Regents, The University Of Texas System Polyamine modified particles
BRPI0513500C8 (pt) 2004-07-19 2022-06-14 Robert Johan Jozeph Hageman Uso de equivalentes de aspartato e composição nutricional ou farmacêutica
DE102004035808A1 (de) 2004-07-21 2006-03-16 Kasch, Helmut, Dr. Ammoniumsalze und Ammoniumsalz-Mineralsalzchlatrate als Transport- und Wirkform für pharmazeutische-medizinische und als Phasentransfermittel für chemische Anwendungen
US8569277B2 (en) 2004-08-11 2013-10-29 Palo Alto Investors Methods of treating a subject for a condition
US20080214440A1 (en) 2004-10-08 2008-09-04 Forbes Medi-Tech (Research), Inc. Vasoactive intestinal polypeptide compositions
US20070293429A1 (en) 2004-10-08 2007-12-20 Therapei Pharmaceuticals, Inc. Vasoactive Intestinal Polypeptide Compositions
US7985418B2 (en) 2004-11-01 2011-07-26 Genzyme Corporation Aliphatic amine polymer salts for tableting
ITME20040015A1 (it) 2004-12-07 2005-03-07 Vincenzo Savica Chewing gum, caramelle gommose, pastiglie, compresse a lento rilascio di chelanti fosfato e/o fosforo salivare e capsule a lento rilascio di chelanti fosfato e/o fosforo a livello gastroenterico.
AU2006264407B2 (en) 2005-07-04 2012-08-30 Ramu Krishnan Improved drug or pharmaceutical compounds and a preparation thereof
HUE025264T2 (en) 2005-08-18 2016-02-29 Panion & Bf Biotech Inc Pharmaceutical-grade ferric citrate for medical use
US8986669B2 (en) 2005-09-02 2015-03-24 Genzyme Corporation Method for removing phosphate and polymer used therefore
WO2007038801A2 (en) 2005-09-30 2007-04-05 Ilypsa, Inc. Monovalent cation-binding compositions comprising core-shell particles having crosslinked poly-vinylic shells, and methods of use thereof
WO2007038802A2 (en) 2005-09-30 2007-04-05 Ilypsa, Inc. Methods for preparing core-shell composites having cross-linked shells and core-shell composites resulting therefrom
EP1928476A1 (en) 2005-09-30 2008-06-11 Ilypsa, Inc. Methods and compositions for selectively removing potassium ion from the gastrointestinal tract of a mammal
WO2007055044A1 (ja) 2005-11-08 2007-05-18 Ajinomoto Co., Inc. 麻酔覚醒促進剤
CA2626734A1 (en) 2005-11-08 2007-05-18 Genzyme Corporation Magnesium-containing polymers for the treatment of hyperphosphatemia
ITMI20052461A1 (it) 2005-12-22 2007-06-23 Univ Degli Studi Milano Sistemi microparticellari per la somministrazione orale di sostanze biologicamente attive
RU2008136081A (ru) 2006-02-14 2010-03-20 Тева Фармасьютикл Индастриес Лтд. (Il) Фармацевтические составы с алифатическими аминными полимерами и способы их производства
EP2016114A2 (en) 2006-05-05 2009-01-21 Genzyme Corporation Amine condensation polymers as phosphate sequestrants
JP2009542653A (ja) 2006-07-05 2009-12-03 ジェンザイム コーポレーション リン酸塩過剰血症のための鉄(ii)含有治療剤
US20100124542A1 (en) 2006-07-18 2010-05-20 Genzyme Corporation Amine dendrimers
CA2660029A1 (en) 2006-08-04 2008-02-07 Nastech Pharmaceutical Company Inc. Compositions for intranasal delivery of human insulin and uses thereof
WO2008027551A2 (en) 2006-09-01 2008-03-06 Genzyme Corporation Dendrimer compositions
US7964182B2 (en) 2006-09-01 2011-06-21 USV, Ltd Pharmaceutical compositions comprising phosphate-binding polymer
JP2010502590A (ja) 2006-09-01 2010-01-28 ユーエスヴィー リミテッド セベラマー塩酸塩およびその処方物の調製のためのプロセス
EP2059247A1 (en) 2006-09-06 2009-05-20 Sucampo AG Method and composition for promoting gastrointestinal bicarbonate secretion
EP2066293A2 (en) 2006-09-29 2009-06-10 Genzyme Corporation Amide dendrimer compositions
BRPI0720234A2 (pt) 2006-12-14 2013-12-24 Genzyme Corp Composição farmacêutica
US20100129309A1 (en) 2007-02-23 2010-05-27 Dhal Pradeep K Amine polymer compositions
US20080207766A1 (en) 2007-02-27 2008-08-28 Agi Therapeutics Research Ltd. Methods and compositions for treating at least one upper gastrointestinal symptom
US20100196305A1 (en) 2007-03-08 2010-08-05 Dhal Pradeep K Sulfone polymer compositions
TWI445540B (zh) 2007-04-20 2014-07-21 Ajinomoto Kk 抗低體溫組成物
JP2010525061A (ja) 2007-04-27 2010-07-22 ゲンズイメ コーポレーション アミドアミンデンドリマー組成物
US8273384B2 (en) 2007-07-02 2012-09-25 Stephen Ray Wurzberger Process for the preparation of a non-corrosive base solution and methods of using same
EP2168992A1 (en) 2007-07-11 2010-03-31 Toray Industries, Inc. Crosslinked polyallylamine or acid addition salt thereof, and use thereof for medical purposes
EP2016947A1 (en) * 2007-07-17 2009-01-21 Chemo Ibérica, S.A. Novel one step process for preparing cross-linked poly(allylamine) polymers
WO2009023544A2 (en) 2007-08-10 2009-02-19 Ilypsa, Inc. Dosage unit anion-exchange polymer pharmaceutical compositions
US20090156647A1 (en) 2007-12-12 2009-06-18 Iovate T. & P. Inc. Method for maintaining physiological pH levels during intensive physical exercise
PA8807201A1 (es) 2007-12-14 2009-07-23 Genzyme Corp Composiciones farmaceuticas
US20100316589A1 (en) 2007-12-14 2010-12-16 Hitesh Bhagat Coated Pharmaceutical Compositions
WO2009097127A1 (en) 2008-01-31 2009-08-06 Genzyme Corporation Pharmaceutical compositions
EA201071059A1 (ru) 2008-03-11 2011-04-29 Лайвайонекс Инк. Способы и композиции для лечения воспаления и связанных с воспалением патологических состояний
WO2009125433A2 (en) 2008-04-08 2009-10-15 Usv Limited Process for preparation of amine polymer salt
US20110142952A1 (en) 2008-06-20 2011-06-16 Harris David J Pharmaceutical Compositions
DE102008030046A1 (de) 2008-06-25 2009-12-31 Ratiopharm Gmbh Kompaktiertes Polyallylamin-Polymer
US20100008988A1 (en) 2008-07-14 2010-01-14 Glenmark Generics, Ltd. Tablet compositions of amine polymers
UY32030A (es) 2008-08-06 2010-03-26 Boehringer Ingelheim Int "tratamiento para diabetes en pacientes inapropiados para terapia con metformina"
WO2010022381A1 (en) 2008-08-22 2010-02-25 Relypsa, Inc. Treating hyperkalemia with crosslinked cation exchange polymers of improved physical properties
US8337824B2 (en) 2008-08-22 2012-12-25 Relypsa, Inc. Linear polyol stabilized polyfluoroacrylate compositions
CN102223790B (zh) 2008-09-25 2015-11-25 维乌作物保护有限公司 生产聚合物纳米颗粒的方法和活性成分的制剂
US20110268666A1 (en) 2008-09-29 2011-11-03 Yissum Research Development Company of the Research University of Jerusalem, Ltd. Novel gastroretentive delivery system
US20100113479A1 (en) 2008-10-30 2010-05-06 Anusuya Choudhury Process for the preparation of tri-substituted pyridine and tri-substituted pyrimidine derivatives useful as gdir agonists
US20100166861A1 (en) 2008-12-29 2010-07-01 Kelly Noel Lynch Pharmaceutical formulations of sevalamer, or salts thereof, and copovidone
RU2011134847A (ru) * 2009-01-22 2013-02-27 Юсв Лимитед Фармацевтические композиции, содержащие фосфатсвязывающий полимер
CA2777682C (en) 2009-10-13 2015-02-24 The Regents Of The University Of Michigan Dendrimer compositions and methods of synthesis
DK2490675T3 (en) 2009-10-22 2019-04-29 Synthon Bv Pharmaceutical compositions with sevelamer
WO2011071927A2 (en) 2009-12-07 2011-06-16 Ironwood Pharmaceuticals, Inc. Treatments for gastrointestinal disorders
JP5964247B2 (ja) 2010-02-24 2016-08-03 レリプサ, インコーポレイテッド 胆汁酸捕捉剤として使用するためのポリイミダゾール
CA2790999C (en) 2010-02-24 2019-05-14 Relypsa, Inc. Crosslinked polyvinylamine, polyallylamine, and polyethyleneimine for use as bile acid sequestrants
IT1406068B1 (it) * 2010-07-22 2014-02-06 Medestea Int Spa Polidesossiribonucleotidi (pdrn) per l'impiego nel trattamento di condizioni di acidosi e composizioni a base di polidesossiribonucleotidi per il suddetto impiego
US20130156720A1 (en) 2010-08-27 2013-06-20 Ironwood Pharmaceuticals, Inc. Compositions and methods for treating or preventing metabolic syndrome and related diseases and disorders
KR101238210B1 (ko) 2011-06-30 2013-03-04 엘지전자 주식회사 이동 단말기
US20130137772A1 (en) 2011-11-29 2013-05-30 Raymond J. Bergeron Hydroxypolyamine salts
SG10201805177PA (en) 2012-06-21 2018-07-30 Keryx Biopharmaceuticals Inc Use of ferric citrate in the treatment of chronic kidney disease patients
CN119405686A (zh) 2012-10-08 2025-02-11 维福(国际)有限公司 治疗高血压和高血钾症的钾结合剂
JP2016535780A (ja) 2013-11-04 2016-11-17 ケリク バイオファーマシューティカルス, インコーポレーテッド 慢性腎臓病患者の心不全を軽減するためのクエン酸第二鉄
PL3229816T3 (pl) 2014-12-10 2020-09-21 Tricida Inc. Polimery wiążące protony do podawania doustnego
EP3452028A4 (en) 2016-05-06 2020-04-15 Tricida Inc. COMPOSITIONS AND METHOD FOR TREATING ACID-BASED DISORDERS
US10934380B1 (en) 2017-09-25 2021-03-02 Tricida, Inc. Crosslinked poly(allylamine) polymer pharmaceutical compositions
AU2018360867B2 (en) 2017-11-03 2024-12-12 Tricida, Inc. Compositions for and method of treating acid-base disorders
AU2018360868B2 (en) 2017-11-03 2025-01-02 Tricida, Inc. Method of treating acid-base disorders
CA3102765A1 (en) 2018-06-04 2019-12-12 Tricida, Inc. Method of treating acid-base disorders
WO2019236639A1 (en) 2018-06-04 2019-12-12 Tricida, Inc. Method of treating acid-base disorders
WO2019236124A1 (en) 2018-06-04 2019-12-12 Tricida, Inc. Method of treating acid-base disorders
US20200306209A1 (en) 2019-03-27 2020-10-01 Tricida, Inc. Method of treating acid-base disorders

Patent Citations (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20160074430A1 (en) * 2013-06-05 2016-03-17 Tricida, Inc. Proton-binding polymers for oral administration

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US11738041B2 (en) 2014-12-10 2023-08-29 Renosis, Inc. Proton-binding polymers for oral administration
US11406661B2 (en) 2016-05-06 2022-08-09 Tricida, Inc. HCl-binding compositions for and methods of treating acid-base disorders
US11992501B2 (en) 2016-05-06 2024-05-28 Renosis, Inc. Compositions for and methods of treating acid-base disorders
US11986490B2 (en) 2017-11-03 2024-05-21 Renosis, Inc. Compositions for and method of treating acid-base disorders

Also Published As

Publication number Publication date
MA54925A (fr) 2021-12-22
CN109414453A (zh) 2019-03-01
JP2022106914A (ja) 2022-07-20
US11406661B2 (en) 2022-08-09
EP3452057A1 (en) 2019-03-13
US20220062328A1 (en) 2022-03-03
WO2017193024A9 (en) 2018-11-22
EP3452028A4 (en) 2020-04-15
SG11201809605PA (en) 2018-11-29
US20190209607A1 (en) 2019-07-11
MA44886A (fr) 2019-03-13
IL308673A (en) 2024-01-01
CN109414453B (zh) 2023-02-17
WO2017193024A1 (en) 2017-11-09
US20250009785A1 (en) 2025-01-09
CN116211887A (zh) 2023-06-06
MY197091A (en) 2023-05-24
AU2023202111A1 (en) 2023-05-04
EP3452028A1 (en) 2019-03-13
CA3023264A1 (en) 2017-11-09
AU2017261337A1 (en) 2018-11-15
KR102655774B1 (ko) 2024-04-05
US20190134076A1 (en) 2019-05-09
MA44875A (fr) 2019-03-13
BR112018072714A2 (pt) 2019-02-19
EP3831395A1 (en) 2021-06-09
JP2025157428A (ja) 2025-10-15
MX2018013476A (es) 2019-03-28
US11992501B2 (en) 2024-05-28
RU2018142943A (ru) 2020-06-08
WO2017193064A1 (en) 2017-11-09
AU2025217383A1 (en) 2025-09-04
IL262660B1 (en) 2023-12-01
IL262660B2 (en) 2024-04-01
JP7071284B2 (ja) 2022-05-18
RU2018142943A3 (enExample) 2020-08-10
IL262660A (en) 2018-12-31
KR20180133931A (ko) 2018-12-17
WO2017193050A1 (en) 2017-11-09
JP2019514965A (ja) 2019-06-06
US20210205351A1 (en) 2021-07-08
AU2023202111B2 (en) 2025-05-15

Similar Documents

Publication Publication Date Title
US11992501B2 (en) Compositions for and methods of treating acid-base disorders
US20250222021A1 (en) Method of treating acid-base disorders
US11986490B2 (en) Compositions for and method of treating acid-base disorders
US20210106611A1 (en) Method of treating acid-base disorders
WO2019236124A1 (en) Method of treating acid-base disorders
US20200306209A1 (en) Method of treating acid-base disorders
HK40055721A (en) Compositions for treating acid-base disorders
NZ787487A (en) Compositions for and method of treating acid-base disorders

Legal Events

Date Code Title Description
AS Assignment

Owner name: TRICIDA, INC., CALIFORNIA

Free format text: ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNORS:KLAERNER, GERRIT;CONNOR, ERIC F.;GBUR, RANDI K.;AND OTHERS;SIGNING DATES FROM 20171010 TO 20180220;REEL/FRAME:047412/0198

STPP Information on status: patent application and granting procedure in general

Free format text: APPLICATION DISPATCHED FROM PREEXAM, NOT YET DOCKETED

STPP Information on status: patent application and granting procedure in general

Free format text: NON FINAL ACTION MAILED

STPP Information on status: patent application and granting procedure in general

Free format text: RESPONSE TO NON-FINAL OFFICE ACTION ENTERED AND FORWARDED TO EXAMINER

STCV Information on status: appeal procedure

Free format text: NOTICE OF APPEAL FILED

STCB Information on status: application discontinuation

Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION

AS Assignment

Owner name: RENOSIS, INC., TEXAS

Free format text: ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNOR:TRICIDA, INC.;REEL/FRAME:063187/0001

Effective date: 20230309

Owner name: RENOSIS, INC., TEXAS

Free format text: ASSIGNMENT OF ASSIGNOR'S INTEREST;ASSIGNOR:TRICIDA, INC.;REEL/FRAME:063187/0001

Effective date: 20230309