CA2185661C - Novel iron chelator and inhibitor of iron-mediated oxidation - Google Patents

Novel iron chelator and inhibitor of iron-mediated oxidation Download PDF

Info

Publication number
CA2185661C
CA2185661C CA002185661A CA2185661A CA2185661C CA 2185661 C CA2185661 C CA 2185661C CA 002185661 A CA002185661 A CA 002185661A CA 2185661 A CA2185661 A CA 2185661A CA 2185661 C CA2185661 C CA 2185661C
Authority
CA
Canada
Prior art keywords
group
daltons
composition
iron
masses
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.)
Expired - Fee Related
Application number
CA002185661A
Other languages
French (fr)
Other versions
CA2185661A1 (en
Inventor
Lawrence Horwitz
Marcus A. Horwitz
Bradford W. Gibson
Joseph Reeve
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.)
University of California
Original Assignee
University of California
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
Priority claimed from US08/383,180 external-priority patent/US5721209A/en
Application filed by University of California filed Critical University of California
Publication of CA2185661A1 publication Critical patent/CA2185661A1/en
Application granted granted Critical
Publication of CA2185661C publication Critical patent/CA2185661C/en
Anticipated expiration legal-status Critical
Expired - Fee Related legal-status Critical Current

Links

Landscapes

  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)

Abstract

Exochelins can be used to prevent damage to living tissue from the formation or presence of the (OH) radical. In particular, the invention is directed to the administration of exochelins to infarcted myocardium prior to or coincidental with reperfusion to prevent damage to myocardium from iron mediated free radical formation. Also presented is the chemical structure of exochelins and modified exochelins at well as other applications of these materials in the treatment and diagnosis of disease in mammals.

Description

WO 96123502 2 ~ ~ ~ 6 6 ~ PCT/1896/OOi7i NOVEL IRON CHELATOR AS INHIBITOR OF IRON-MEDIATED OXIDATION
This invention was made in part with government support from NIH Grant AI-33790 and NIH Grant HL-48177.
The present invention relates to the chemical structure of a previously unidentified series of high affinity, iron-binding compounds, referred to by prior investigators as exochefins, which are released by mycobacteria. The invention also relates to modifications to these newly identified compounds to vary their physiological properties and applications of these newly identified and modified compounds.
!n acute myocardial infarction, cardiac tissue is damaged by two sequential events, hypoxia in the ischemic phase and oxidative damage in the reperfusion phase. Myocardium damaged in the ischemic phase can be salvaged by reintroduction of blood to the ischemic area.
However, reperfusion can result in injury as a result of an inflammatory response in the reperfused tissue caused by the migration of leukocytes into the tissue and the production of reactive oxygen species. One of the most reactive species is the hydroxyl species (OOH) which is generated in the presence of iron and which results in cell death. Prevention of the formation of (OOH) will prevent lethal cell damage from this cause. It is known that the formation of (OOH) is dependent on the presence of free iron and that iron chelators will prevent reperfusion injury. For example, the iron cheiators deferoxamine, when administered prior to reperfusion, prevent injury and reduces myocardial infarct size during coronary artery occlusion and reperfusion. However, reperfusion injury occurs rapidly after the reestablishment of blood flow to the ischemic myocardium.
The formation of the (OOH) radical is dependent on the presence of free iron; iron chelators can scavenge the free iron and thus suesrlrurE sHE~r ~~uu ~
2 ~., , PC1'IiB96100171 render the iron unavailable to catalyze the hydroxyl radical formation.
However, these prior known iron chelating materials either do not prevent (OOH) production by the Fenton reaction (i.e., EDTA), or enter the cells too slowly (i.e., desferoxamine) such that sufficient quantities are not' available to act rapidly enough to chelate enough iron to prevent the formation of (OOH) and the subsequent cell destruction. Desferoxamine has been demonstrated to be effective if administered prior to occurrence of the myocardial infarct but to be ineffective if administered at or after the onset of reperfusion.
Similar injury to heart tissue can occur as a result of heart bypass procedures, such as during open heart surgery, or to other body organs when they are deprived of oxygenated blood as a result of surgery or injury.
Exochelins were briefly described and their general function in the growth of mycobacteria was discussed by Macham, Ratledge and Barclay at the University of Hull in England (Lionel P. Macham, Coffin Ratledge and Jennifer C. Nocton, "Extracellular Iron Acquisition by Mycobacteria: Role of the Exochelins and Evidence Against the Participation of Mycobactin", Infection and Immunity, Vol. 12 No. 6, p.
1242-1251, Dec. 1975; Raymond Barciay and Colin Ratlege, "Mycobactins and Exochelins of Mycobacterium tuberculosis, M. bovis, M. africanum and Other Related Species", Journal of General Microbioloov, 134, 771-776, (1988); L.P. Macham and C. Ratledge, "A
New Group of Water-soluble Iron-binding Compounds from Mycobacteria:
The Exochelins", Journal of General Microbioloov, 89, 379-282, (1975)).
Macham identified the existence of a substance found in the extracellular fluid, which he referred to as exochelin. He described exochelin as a water and chloroform soluble compound which has the ability to chelate free iron. According to Macham, this material has similarities to W096123502 218 5 6 61 P~~96IOOI7i
3 mycobactin, which is located in the cell wall and functions to transmit iron to the interior of the cell. However, in contrast thereto, mycobactin is a lipophilic, water insoluble molecule which is unable to diffuse into, and assimilate free iron from, the extracellular environment. Macham et al recognized that exochelin functions at physiological pH to sequester iron from other iron bearing compounds in the serum, such as transferrin or ferritin, and present the iron in a form that can be transferred to mycobactin. Macham et al. did not isolate or purify the exochelins but identified them as a yenta- or hexapeptide, having a molecular weight of 750 to 800, containing 3 mol of s-N-hydroxylysine, sN-acetyl-sN-hydroxylysine, or eN-hydroxyornithine and 1 mol of threonine. Also, depending on the bacterial source of the exochelin, he disclosed that the molecules may also include ,B-alanine or salicylic acid.
Barcfay (ibid) described the production of exochelins from twenty-two different strains of M, tuberculosis and related species.
However, these prior investigators did not determine the specific structure of exochelins or identify any applications of the exochelins other than their function as a transport medium for iron to mycobactin located in the cell wall.
Thus there is a need for a substance that can be easily administered at the time of reperfusion and which will rapidly chelate the free iron as it is formed or made available to prevent the formation of the (OOH) radical. Further, there is a need to identify the specific structure of exocheline so that its function can be more fully understood and its utility as a diagnostic, treatment and preventive modality can be elucidated.

Cardioplegia solutions are used during cardioplegia procedures, which is a procedure where the cardiac mechanical activity is temporarily halted.
Cardioplegia solutions ere described in "Cardiopulmonary Bypass: Principles and Techniques of Extracorporeal Circulation" (1995 edition) - Chapter 2 pp. 21-39, the requirements of cardioplegic solutions are to: (a) induce myocardial diastolic relaxation (arrest); (b) maintain a favorable metabolic mi~_ieu; (c) prevent interstitial and intracellular edema; (d) prevent loss of cellular metabolites; (e) maintain appropriate acid-base balance: and (f) provide metabolic substrate (oxygen and glucose).
The Inova Health System explains that when a patient is placed on the heart-lung machine, the heart and body are cooled to reduce the heart's metabolic requirements and oxygen consumption. Coi.d chemical agents such as potassium chloride can be infused into the heart to further reduce the metabolic requirements and oxygen consumption of the heart by quickly causing the heart to stop beating, causing cardioplegia (cardiac paralysis). Without these chemical agents, the heart will continue to quiver or remain in a state of ventricular fibrillation while the surgery takes place. This situation wastes energy resources in the heart that can be used when t:he heart needs to be stimulated to start beating again.
Cardioplegia, or cardiac paralysis, allows the surgeon to perform delicate procedures on a motionless heart. The chemical agents are rei.nfused into the heart periodically, in a solution of axyger~ated blood. Thus, repeat infusions of blood cardioplegia solution provide oxygen to the heart while it remains at a standstill or arrest.

SUMMARY
In accordance with one aspect of the present invention there is provided a composition, for protecting live tissue in a mammal from injury resulting from exposure to the hydroxyl free radical formed following re-establishment of fluid flow to a body organ after restriction of blood flow to that body organ, the composition comprising in combination an effective amount of at least one water and lipid soluble desferriexochelin, and a pharmaceutically acceptable carrier, wherein the amount of desferriexochelin is sufficient to protect the mammal on re-establishment of flow of fluid to the tissue.
Another aspect of the present invention provides for the use of exochelins to prevent damage to living tissue from the formation or presence of the (OOH) radical. In particular, this aspect of the invention is directed to the administration of exochelins to infarcted myocardium prior to or coincidental with reperfusion to prevent damage to myocardium from iron mediated free radical formation. Also presented is the chemical structure of exochelins and modified exochelins as well as other applications of these materials in the treatment and diagnosis of disease mammals.
T1 T'1 T T.7 T TT l~ C~
These and other features, aspects and advantages of the present invention will become better understood with reference to the following description, appended claims, and accompanying drawings, where:
- 4 -Figure 1 shows the chemical structure of an iron chelate of exochelin (ferriexochelin) and the desferriexochelin (iron free) molecule.
Figure 2 shows an elution profile of a culture filtrate of M. tuberculosis monitored at 220nm and 450nm.
Figure 3 shows an elution profile of the same filtrate monitored at 450nm with the molecular weight of each peak shown.
Figure 4 shows the mass spectrometer spectra of a major serine-containing exochelin at m/z = 720.3 along with the structure determined therefrom.
- 4a -WO96J23502 218 5 b 61 p~J~96100171 Figure 5 is a graph showing the inhibition of cell injury as a result of the use of an exochelin mixture on cardiac myocytes.
Figure 6 is a graph showing the inhibition of cell injury as a
5 result of the use of exochelin 758C on cardiac myocytes.
Figure 7, 8, and 9 are graphs comparing the inhibition of cell injury as a result of the use of exochelin 758C, 772A and 772C on cardiac myocytes.
Figure 10 shows the chemical structure of an iron chelate of exochelin (ferriexochelin) and the desferriexochelin (iron frees molecule with cites for modification identified.
DETAILED DESCRIPTION OF THE INVENTION
It has been found that exochelins can block, or significantly reduce, oxidative damage to tissue resulting from the iron-mediated catalysis of tissue/free radicals reactions, such as the hydroxyl radical t~OH), particularly hydroxyl radicals generated in the Fenton reaction, commonly referred to as reperfusion injury. It has been further found that the exochelins are effective to retard or prevent reperfusion injury when administered at the start of or concurrent with reperfusion. Additionally, it has been found that exochelins encompass a much broader class of materials and have a different chemical structure then originally theorized by Macham et al. and Barclay et al.
It has also been found that these materials can chelate a broad range of metals to result in materials not previously known.
Besides preventing reperfusion injury, properly modified exochelins can be used to treat certain diseases, attack certain cells, such as cancer cells, R'O 96123502 2 '~ PCTIIB96100171
6 and be used to monitor the effectiveness of drug treatment and detect the presence of certain disease states. In particular, it is known that the growth of neuroblastoma cells can be negatively affected by the removal of iron using the iron chelating compound desferrioxamine without similarly affecting the growth of normal cells. Other applications of exochelins include treatment of iron overload from transfusions or cancer chemotherapy, particularly for leukemia.
As a result of isolating and purifying exochelins, it has been found that exochelins are a family of molecules having a range of molecular weights and various different side chains. Further, purified exochelins have been prepared and their utility as scavengers of free iron, such that they are effective in preventing the formation of tissue damaging hydroxyl radicals (OOH), has been demonstrated for the first time. In particular, purified exochelins of M. tuberculosis have been isolated and have been shown to effectively remove iron from transferrin, lactoferrin and ferritin at physiological pH without transmitting any of the infectious properties of the bacteria from which they are derived. It has also been demonstrated for the first time that these exochelins block hydroxyl radical formation by the Fenton reaction and, based on the response of cardiac myocytes, can be effective to prevent reperfusion injury after myocardial infarction or vascular insults to other tissue when administered after the attach occurs as well as for several hours after the episode.
While mycobactins have been extensively studied, individual exochelins had not been isolated or purified and their structure and composition had not been previously defined. Further, we have found that prior references have mischaracterized the exochelins, and thus have failed to identify the structure of these compounds. In particular, Macham (ibid.) identified them as a penta- or hexapeptide, having a WO 96!23502 - ~ ~ ~ ~ p~/Ig96100I~I
molecular weight of 750 to 800, containing 3 mol of e-N-hydroxylysine, sN-acetyl-eN-hydroxylysine, or sN-hydroxyornithine and 1 mol of threonine. We have found that the exochelins have a much broader range of molecular weights, constitute several series of compounds with an identifiable difference in molecular weights, include only 2 mol of s-N-hydroxylysine and are not peptides. A peptide is a polymer of an amino acid (NHz CHR-COOH) formed by the condensation of the carboxylic group of a first molecule with the amino group of another molecule to form an amide linkage (-CO-NH-). Exochelins cannot be considered to be peptides. Instead, they contain three amino acids and other structural moieties (salicylic acid, dicarboxylic acids or monoester analogs, and hydroxy carboxylic acids) formed by amide (-NH-CO-), hydroxymate (-NH(OH)-CO-) and ester condensations (-CO-O-). The ferri- and desferri forms are shown in Figure 1.
Preparation - Exochelins were generated and purified from a virulent (Erdman) and avirulent (H37Ra) strain of M. tuberculosis. To enhance the production of M. tuberculosis exochelins the bacteria were cultured in an iron deficient medium. In particular, the Erdman strain of M. tuberculosis (American type culture collection 35801 ) and H37Ra (ATCC 25177) were grown on Middlebrook 7H11 agar plates at 37°C in 596 COa. After 14 days the bacteria were harvested, suspended in 150 ml of modified Sauton's medium in culture flasks and incubated for 3 to 8 weeks. The modified Sauton's medium contained 0.12 mg/I ferric ammonium citrate without added surfactant.
Iron rich exochelins (ferriexochelins) were then recovered by filtering, saturating with iron and extracting with chloroform and purified by high pressure liquid chromatography (HPLC): Specifically, the supernatant fluid from the above suspension was filtered through successive 0.8pm and O.ZUm low-protein binding filters. The exochelins wo ~soz pcr~9~oom were then loaded with iron by saturating the filtered supernatant fluid by exposure to ferric chloride (150mg per liter of culture filtrate). The ferric-exochelins were mixed with chloroform (1 volume of culture filtrate per 1.5 volumes of chloroform) ancl, after separation of the layers, the exochelin rich chloroform layer was removed and stored under anhydrous magnesium sulfate (2gll). The chloroform extract was then passed through a fritted glass tiller and evaporated by rotary evaporation leaving behind a brown residue.
The brown residue was further purified by suspension in 5ml of a first buffered solution (0.1 % trifluoroacetic acid) which was introduced into a liquid chromatography column (C-18 Sep-Pal' cartridge).
The brown band which formed near the top of the column was eluted with a second buffer (0.1 % TFA, 50% acetonitrile). The partially purified material was then diluted three-fold in 0.1 % trifluoroacetic acid and subjected to reverse phase high pressure liquid chromatography at a rate of 1 mllmin followed by exposure to a C-18 column. The presence of the iron rich exochelins in the HPLC eluate was detected by simultaneous monitoring of the UV absorbance of the 450nm peak (iron compounds) and the 220nm peak which is indicative of amide and aromatic groups.
Approximately 5 major and 10 minor peaks, shown in Figure 2, eluted out of the final C-18 column exhibited a high 4501220nm absorbance ratio.
These were confirmed to be exochelins by mass spectrometry. Major peaks were further purified by a second reverse phase HPLC on an alkyl-phenyl column. The exochelins recovered from the Erdman strain of M.
tuberculosis were identical to the exochelins recovered from the H37Ra strain.
Characterization - Based on LSIMS and ESI-MS analysis of the numerous peaks, in their ferri- (Fe3+) form, eluted from the column (see Fig. 3), the iron-exochelins are not confined to the two specific * - Trade Mark 1 W096123502 PCT'/IB96/OOI71 molecules detailed above but include a family of species ranging in mass from 716 to 828 daltons. Each member of the family appears to differ from its neighbor by 14 daltons, reflecting the number of CH2 groups in the R~ alkyl side chain andlor 2 daltons, reflecting the presence of a double bond in the R, alkyl side chain. Accordingly, the exochelins appear to form two series with the subsequent members of each series differing in mass by 14 daltons, the saturated series having masses of approximately 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series having masses of 742, 756, 770, 784 798, 812 and 826. Additionally, the presence or absence of a methyl group at R3 (i.e., H or CH3) further defines an additional two series of molecules referred to as the serine (R3=H) and the threonine series (R3=CH3), as confirmed by amino acid analysis. The most polar compounds are to the left of the figure (elute earlier) and the least polar (most soluble in lipid) are to the right. However all the peaks are water soluble. Where more than one peak was found to have the same molecular weight each peak is further designated A, B or C (i.e., 758A, B and C) to indicate the level of polarity with A representing the more polar compound and the C
representing the less polar form. The more polar forms are believed to result from a methyl groups attached at different location in the molecule.
Structure of the Exochelin - Figure 4 shows the results of tandem mass spectrometric analysis under induced dissociation (He floated at 2 keV for a collision energy of 6 keV) of the major saturated serine-containing desferriexochelin with (M+H)* at mlz 720.3. The fragment ions were assigned to one of the six structural moieties A-F
resulting from the cleavage products generated about the amide or ester bonds with the hydrogen transfer relative to the neutral molecule - associated with each peak indicated on the spectrum shown in Figure 4.
Acid hydrolysis and methylation of the exochelins resulted in the formation of salicylic acid and pimelic acid. The mass spectrographic R'O 96~23s~? 21 8 5 6 6 1 FCT/DB96100t7t ,o analysis indicates that the pimelic acid is present in the exochelin as a methyl ester.
Based on this analysis the general structure of the ferriexochelins and the desferriexochelins is shown in Figure 1. The methyl group shown at the RQ position (as defined in Figure 10) may be in the RS position. The iron-exochelin core molecule is circular with iron in the center. It contains 3 amino acid moieties (two N-hydroxylysines and 1 serine or threonine, depending on whether R3 is a hydrogen or methyl group). The major difference between exochelins and mycobactins of M.
tuberculosis is that R, in the exochelins exists as either a saturated adkyi methyl ester ((CH2)NCOOCH3) or a singly unsaturated alkyl methyl ester (CHz)xCH=CH(CHa)YCOOCH3 and exochelins have a much shorter alkyl side chain than mycobactins with these shorter side chains terminating in methyl ester moieties. These differences provide for the water solubility of the exochelins and their ability to function in the extracellular environment.
Clinical Utility - The clinical utility of the administration of exochelins to prevent reperfusion injury was demonstrated by application to adult rat myocytes.
In the Examples below the different exochefins, in both the desferri- and fern- form, will be identified by the molecular weight as shown in the elution curve in Figure 3.
Example 1 The heart of a male rat was excised after the rat was anesthetized, a thoracotomy performed and the heart chilled in situ. The excised heart was then placed on a Langendorff apparatus and perfused with a collagenase and hyaiuronidase in a 50pM calcium in modified Krebs wo 96n3soZ pcr~moom Ringer buffer solution. The tissue was then finely divided and dispersed in a collagenase/trypsin solution, filtered into a cold trypsin inhibitor solution and exposed to increasing concentrations of calcium. After removal of damaged cells, the remaining cell suspension was placed in 5 several larninin-coated plastic dishes along with a culture medium containing 5% fetal bovine serum.
After the cultures were allowed to sit for 48 hours hydrogen peroxide was added to each dish and the lactate dehydrogenase activity (LDH), which is indicative of cell injury, was measured at variaus time intervals. A cell injury index (CII) for comparison purposes was obtained by measuring the LDH in a nonexposed cell culture in both an as is condition (0 Index) and following exposure to a detergent that lysis 100%
of the myocytes (1% Tritori X-100) representing a CII of 100. The LDH
15 under specified treatment conditions for various periods of time was then determined, the corresponding CII value determined and the individual results were plotted against time (Figure 5).
Using the procedure described above, a mixture of the desferri- farm of exochelins 772C and 784 (a 50:50 mixture of the 772C
peak and the 784 peak), a relatively non-polar substance, was isolated and used to treat cell cultures. The exochelin were converted to the desferriexochelin form by incubation for several days with 50 millimolar EDTA at pH 6. The desferri- form was then repurified by chloroform extraction.
Three samples of cells were exposed to either a) H202, b) H202 and 50,uM of desferriexochelin (iron free exochelin) added simultaneously or c) H~OZ added 2 hours after addition of 100,uM of 30 desferriexacheiin to the cell culture (preincubation). The untreated cell cultured showed almost 62% cell injury over a 4 hour period. In contrast - Trade Mark wo 96I23soz 218 5 6 61 PCTIIB96100171 thereto, addition of exochelin simultaneously with, or 2 hours prior to, peroxide addition substantially prevented or significantly reduced cell damage, the cell injury being approximately 2 to 9%.
~xamole 2 The procedure of Example 1 was repeated with desferri -exochelin 758C which is relatively more polar than exochelins 772C and 784. There was tittle or no difference between the effect when desferriexochelin 758C was delivered along with or within 15 minutes of delivery of H,Oz. In both instances after 2 hours the cell destruction was substantially the same as in the control. However, delivery of the desferriexochelin 758C 2 hours prior to H20z introduction cut the cell destruction to a CII of about 20. The results are shown in Figure 6.
Example 3 The procedure set forth above was repeated using desferriexochetin 772A, 772C and 758C. Plotted in Figures 7 - 9 are the results for 2 hour predelivery, simultaneous delivery and 20 minute delayed delivery of the exochelins. Only exochelin 772C shows retardation of injury under all conditions while exochelin 772A is not effective under any conditions. On the other hand, exochelin 758C
shows protection only if delivered 2 hours prior to peroxide introduction.
It is therefor concluded that the relatively non-polar, more lipid soluble exochelins are effective when administered with or after formation of the (OOH) radical, i.e., after injury occurs; the more polar exochelins must be administered 1 to 2 hours prior to the free radical generating event to prevent or reduce cell destruction.

wo vsra.~soa 218 5 6 6 i P~~~~~t71 Example 4 The capacity of exochelins to compete for iron with host iron-binding proteins was determined by incubating desferriexochelin with solutions of transferrin, lactoferrin, or ferritin at 4:1 and 1:1 molar ratios of iron to exocheiin. The conversion of the exochelin from its desferri- to its ferri- form was then determined by reverse phase HPLC. Within one minute of exposure of desferriexochelin to 95% iron-saturated transferrin, the exochelin had started to pick up iron from the transferrin and within one hour the exochelin was fully saturated with iron. Iron was also readily removed from 40% iron-saturated transferrin, which approximates the iron level in transferrin as it exists in serum. Similar results were obtained when desferriexochelin was exposed to iron-saturated lactoferrin. Likewise, ferritin released iron to the exochelin but at a slower rate than other iron binding proteins.
It has been discovered that exochelins are very effective in scavenging free iron in a physiological system and withdrawing iron from iron bearing protein. In particular it has been found that exochelin effectively block the formation of the hydroxyl free radical (OOH) and thus significantly reduce or prevent the injury to ischemic tissue when circulation of blood to that tissue is reestablished with the higher molecular weight, less polar exochelins being more effective in preventing cell destruction. While the benefit to cardiac tissue has been demonstrated, the benefit of the use of exochelins following interruption of blood flow to other body organs, including but not limited to the brain, kidney, liver, bowel, and skeletal muscle is now apparent.
Experimentation has shown that the affinity of the exochelins is not limited to iron but that other metals can be chelated, such as Na, K, Mn, Mg, AI and Zn. Therefore, the exochelins can be used to deliver to the body various desirable metals or chelate various WO96/23502 21' O 5 U 6 PCTIIB96100171 undesirable metals within the body. Additionally, certain cells, including certain cancer cells are known to have a need for or affinity for certain metals. This can be utilized to deliver to that cell reactive compounds attached to the exochelins for destruction of the cell (chemotherapy) or to target a diseased organ with a beneficial drug bound to the exochelin.
Conversely, since certain cancer cells have a high demand for iron, the desferriexochelins can be used to bind free iron, thus preventing iron delivery to the cancer cell, resulting in the destruction of the cancer cell.
While the structure of exochelins recovered from M.
tuberculosis is shown in Figure 1, it is known that other mycobacteria can generate exochelins and that these exochelins may have different structure and include different amino acids depending on the mycobacteria from which they are derived. However, all exochelins will behave in a similar manner and exist in similar series with subsequent members thereof having a similar progression of molecular weights. The effectiveness of the different members of the series will also depend on the relative polarity of the molecules. Therefore, the invention contemplates exochelins generated from other mycobacteria including, but not limited to, M. tuberculosis, M. microti, M. bovis, M. africanum, M.
kansasii, M. marinum, M. gastri, M. nonchromogenicum, M. terrae, M.
trivale, M. maimoense, M. shimoidei, M. gordonae, M. asiaticum, M.
szulgai, M. simiae, M. scrofulaceum, M. avium, M. intracellulare, M.
xenopi, M. ulcerans, M. haemophilum, M. farcinogenes, M. lepraemurium, M. paratuberculosis, M. chelonae subsp. chelonae, M. chelonae subsp.
abscessus, M. fortuitum, M. chitae, M. senegalense, M. agri, M.
smegmatis, M. phlei, M. thermoresistibile, M. aichiense, M. aurum, M.
chubuense, M. duvalii, M. flavescens, M. gadium, M. givum, M.
komossense, M. neoaurum, M. obuense, M. parafortuitum, M. rhodesiae, M. sphagni, M. tokaiense or M. vaccae.

W096l23502 ~ ~ PCTIIB96/OOI7I
It is also contemplated that exochelins can be modified to effect their solubility properties, metal chelating ability or cellular absorption rates. Additionally, detection of modified exochelins or exochelin in their metal chelated state, using monoclonal antibodies or 5 chemical analysis as diagnostic tools, by blood analysis, urinalysis or noninvasive instrumental techniques, to monitor progress of a disease state or effectiveness of treatment. In particular, referring to the structures of the metal containing and metal free compounds shown in Figure 10, the following substitutions are contemplated:
R, _ (CHZ)"CH3 as a linear or branched chain; (CHz)"COOH, a fatty acid; (CHZ)"COOR, a fatty acid ester where R is an alkyl group;
(CHz)"CONH2;
R2 = a substitution at any of the 4 open ring sites of alkyl groups, sulfonamides, hydroxyl, halogen, acetyl, carbamyl, amines, NOZ or any combination thereof;
R3 - the H (serine) or CH3 (threonine) can be replaced by side chains found on ~-hydroxy amino acids which are capable of forming cyclic oxazofine structures.
R4, and R4b = H, CH3 or other alkyl or substituted alkyl groups;
Rs, and R5b = H, CH3 or other alkyl or substituted alkyl groups;
X = O, NH, S, CHZ;
M = mono-, di-, or trivalent metals such as Pb. Ai, Cd, Ni, Ag, Au, As, Mg, Mn, Zn, Cu, Ru, Nb, Zr, Ta, V, Ga, Pt, Cr, Sc, Y, Co, Ti, Na, K;

R'096/23502 ~'18 5 6 6.1 PCTI1896/00171 ~ represents chiral centers which may be R or S;
The various hydroxyl groups (OH) involved in chelating the metal can be replaced by various functional groups, such as H or a halogen, to vary the affinity of the compound for the chelated metal or to convert the molecule into a metal antagonist.
Although the present invention has been described in considerable detail with reference to certain preferred versions and uses thereof, other versions and uses are possible. For example, exochelins can be used to attack infectious bacteria, such as M. tuberculosis, by blocking access of the mycobacteria to iron, to remove toxic levels of metals from the body or to deliver desirable metals to the body. Further, modified metal containing exochelins can deliver appended active drugs or chemicals to cites in the body which preferentially absorb the chelated metaland preferentially absorbed exochelins with chelated metals can be used as targets for treatment by other modalities, such as microwave energy for hypothermia treatment of cancer cells. Therefore, the spirit and scope of the appended claims should not be limited to the description of the preferred versions contained herein.

Claims (14)

We Claim:
1. A composition, for protecting live tissue in a mammal from injury resulting from exposure to the hydroxyl free radical formed following re-establishment of fluid flow to a body organ after restriction of blood flow to that body organ, the composition comprising in combination an effective amount of at least one water and lipid soluble desferriexochelin, and a pharmaceutically acceptable carrier, wherein the amount of desferriexochelin is sufficient to protect the mammal on re-establishment of flow of fluid to the tissue.
2. A composition, for preventing injury to living tissue in a mammal from the presence of iron mediated hydroxyl radical formation, the composition, together with a pharmaceutically acceptable carrier, comprising an effective amount of at least one desferriexochelin of the formula:
wherein:
R1 is selected from the group consisting of (CH2) n COOCH3 and (CH2) x CH=CH (CH2) y COOCH3, in which n is from 1 to 7, and x+y is from 1 to 5;
R2 is at least one chemical moiety substituted at one or more of the 4 open sites on the ring, and which is a substituent chosen from the group consisting of alkyl groups, sulfonamide group, hydroxyl, halogen, acetyl, carbamyl, amino groups and nitro (NO2) and combinations thereof; and R3 is selected from the group consisting of H and CH3, wherein the compound has a molecular weight of from 663 to 775 Daltons.
3. A desferriexochelin compound having the formula:
wherein:
R1 is selected from the group consisting of (CH2)n COOCH3 and (CH2) x CH=CH(CH2) y COOCH3, in which n is from 1 to 7, and x+y is from 1 to 5;
R2 is at least one chemical moiety substituted at one or more of the 4 open sites on the ring, and which is a substituent chosen from the group consisting of alkyl groups, sulfonamide group, hydroxyl, halogen, acetyl, carbamyl, amino, nitro (NO2) and combinations thereof; and R3 is selected from the group consisting of H and CH3, wherein the compound has a molecular weight of from 663 to 775 Daltons.
4. A composition according to Claim 2 wherein the composition, together with a pharmaceutically acceptable carrier, includes a mixture of desferriexochelins having a molecular weight of from 719 to 731 Daltons.
5. A composition according to Claim 2 wherein the composition, together with a pharmaceutically acceptable carrier, includes a mixture of relatively non-polar desferriexochelins, relative to the remainder of the compounds defined in claim 2, in which n is 5, 6 or 7.
6. A composition according to Claim 2 wherein the composition, together with a pharmaceutically acceptable carrier, includes a mixture of relatively non-polar desferriexachelins, relative to the remainder of the compounds defined in Claim 2, in which x+y is 4 or 5.
7. A composition, for delivering an active compound to a mammal to treat a medical condition caused by the formation of, or presence of, hydroxyl free radicals, the composition comprising a pharmaceutically acceptable carrier together with an effective amount of at least one desferriexochelin compound of the formula:
wherein:
R1 is selected from the group consisting of (CH2) n (CH3), (CH2) n COOH, (CH2) n COOR, (CH2) x CH=CH (CH2) y COOH and (CH2) x CH=CH (CH2) y COOR, or (CH2) n CONH2, wherein R is an alkyl, in the ferri-form the saturated series having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and in the ferri-form the unsaturated series having masses of 742, 756, 770, 784, 798, 812 and 826 daltons, n is from 1 to 7, and x+y is from 1 to 5;
R2 is at least one chemical moiety substituted at one or more of the 4 open sites on the ring, and which is a substituent chosen from the group consisting of alkyl groups, the saturated series having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series having masses of 742, 756, 770, 784, 798, 812 and 826 daltons, sulfonamide group, hydroxyl, halogen, acetyl, carbamyl, amino groups, nitro (NO2) and combinations thereof;
R3 is a chemical moiety chosen from the group consisting of H, CH3, and side chains found on .beta.-hydroxyamino acids which are capable of forming oxazoline structures;
R4a, R4b, R5a and R5b are selected from the group consisting of H
and alkyl groups; and X represents O, NH, S or CH2.
8. An isolated metal chelate having the formula:
wherein:
R1 is a chemical moiety selected from the group consisting of (CH2) n CH3, (CH2) n COOH, (CH2) n COOR, (CH2) x CH=CH (CH2) y COOH, (CH2) x CH=CH (CH2) y COOR, and (CH2) n CONH2, wherein R is an alkyl group, the saturated series having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series having masses of 742, 756, 770, 784, 798, 812 and 826 daltons, n is from 1 to 7 and x+y is 1 to 5;
R2 is at least one chemical moiety substituted at one or more of the 4 open sites on the ring, and is selected from the group consisting of alkyl, the saturated series having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series having masses of 742, 756, 770, 784, 798, 812 and 826 daltons, sulfonamide group, hydroxyl, halogen, acetyl, carbamyl, amino, and nitro (NO2) and combinations thereof;
R3 is a chemical moiety chosen from the group consisting of H, CH3 and side chains found on .beta.-hydroxy amino acids which are capable of forming cyclic oxazoline structures;
R4a, R4b, R5a and R5b are selected from the group consisting of H and alkyl groups; and M is selected from the group consisting of iron, lead, aluminium, cadmium, nickel, silver, gold, arsenic, magnesium, manganese, zinc, copper, rubidium, niobium, zirconium, tantalum, vanadium, gallium, platinum, chromium, scandium, yttrium, cobalt, titanium, sodium and potassium; and X is O, NH, S or CH2.
9. The metal chelate of Claim 8 wherein M is iron.
10. A composition, for protecting live tissue in a mammal from injury resulting from exposure to the hydroxyl free radical formed following re-establishment of fluid flow to a body organ after restriction of blood flow to that organ, which composition comprises a pharmaceutically acceptable carrier together with at least one water and lipid soluble desferriexochelin compound, the amount being effective to protect the live tissue in the mammal upon re-establishment of flow of fluid to the tissue, for administration in a solution selected from a reperfusion solution and a cardioplegia solution.
11. A composition, for protecting live tissue in a mammal from injury resulting from exposure to the hydroxyl free radical formed following re-establishment of fluid flow to a body organ after restriction of blood flow to that body organ, the composition comprising a pharmaceutically acceptable carrier together with an effective amount of at least one desferriexochelin compound of the formula wherein:
R1 is selected from the group consisting of (CH2) n COOCH3 and (CH2) x CH=CH (CH2) y COOH3 in which groups n is from 1 to 7 and x+y is from 1 to 5;
R2 is at least one chemical moiety substituted at one of more of the 4 open sites on the ring, and is selected from the group consisting of alkyl groups, the saturated series, when in the ferr-form having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series, when in the ferri-form of 742, 756, 770, 784, 798, 812 and 826 daltons, sulfonamide group, hydroxyl, halogen, acetyl, carbamyl, amino, nitro(NO2) and combinations thereof; and R3 is H or CH3;
wherein:
(i) the at least one desferrioexochelin compound has a molecular weight of from 663 Daltons to 775 Daltons, (ii) the amount is effective to protect the live tissue upon re-establishment of flow of fluid to the tissue; and (iii) the composition is for administration in a solution selected from the group consisting of a reperfusion solution and a cardioplegia solution.
12. A composition, for delivering an effective amount of at least one desferriexochelin compound to a mammal to treat a medical condition caused by the formation of, or the presence of, hydroxyl free radicals, the composition comprising a pharmaceutically acceptable carrier together with an effective amount of a compound of the formula wherein:
R1 is a chemical moiety selected from the group consisting of (CH2) n CH3, (CH2) n COOH, (CH2) n COOR, (CH2) x CH=CH (CH2) y COOH, (CH2) x CH=CH (CH2) y COOR and (CH2) n CONH2 in which R is an alkyl, the saturated series having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series having masses of 742, 756, 770, 784, 798, 812 and 826 daltons, n is from 1 to 7 and x+y is 1 to 5;
R2 is at least one chemical moiety substituted at one or more of the four open sites on the ring, and is selected from the group consisting of alkyl groups, the saturated series having masses of 716, 730, 744, 758, 772, 786, 800, 814 and 828 daltons and the unsaturated series having masses of 742, 756, 770, 784, 798, 812 and 826 daltons, sulfonamide group, hydroxyl, halogen, acetyl, carbamyl, amino, nitro(NO2) and combinations thereof;
R3 is a chemical moiety selected from the group consisting of H, CH3 and side chains found on .beta.-hydroxyamino acids which are capable of forming cyclic oxazoline structures:
R4a. R4b, R5a and R5b are selected from the group consisting of H and alkyl groups; and X is O, NH, S or CH2;
wherein:
(i) the amount of the at least one desferriexochelin compound is effective to protect the mammal upon re-establishment of flow of fluid to an organ within the mammal: and (ii) the composition for administration in a solution chosen from the group consisting of a reperfusion solution and a cardioplegia solution.
13. A process for obtaining a metal chelate according to Claim 8 which comprises exposing an ion of the metal M in solution to a desferriexochelin.
14. A process according to Claim 13 wherein the metal M is iron.
CA002185661A 1995-02-03 1996-01-26 Novel iron chelator and inhibitor of iron-mediated oxidation Expired - Fee Related CA2185661C (en)

Applications Claiming Priority (3)

Application Number Priority Date Filing Date Title
US08/383,180 US5721209A (en) 1995-02-03 1995-02-03 Iron chelator and inhibitor of iron-mediated oxidant injury
US08/383,180 1995-02-03
PCT/IB1996/000171 WO1996023502A1 (en) 1995-02-03 1996-01-26 Novel iron chelator as inhibitor of iron-mediated oxidation

Publications (2)

Publication Number Publication Date
CA2185661A1 CA2185661A1 (en) 1996-08-08
CA2185661C true CA2185661C (en) 2005-10-04

Family

ID=35395857

Family Applications (1)

Application Number Title Priority Date Filing Date
CA002185661A Expired - Fee Related CA2185661C (en) 1995-02-03 1996-01-26 Novel iron chelator and inhibitor of iron-mediated oxidation

Country Status (1)

Country Link
CA (1) CA2185661C (en)

Also Published As

Publication number Publication date
CA2185661A1 (en) 1996-08-08

Similar Documents

Publication Publication Date Title
AU699916B2 (en) Novel iron chelator and inhibitor of iron-mediated oxidation
EP1021189B1 (en) Desferri-exochelin for the treatment of atherosclerosis and vascular injury by prevention of vascular smooth muscle cell proliferation
JP2000503625A (en) Novel iron chelators as inhibitors of iron-mediated oxidation reactions
JP2001524081A (en) Composition for preservation of living biological material and method of use thereof
JP4709552B2 (en) LFA-1 inhibitor and use thereof
CA2185661C (en) Novel iron chelator and inhibitor of iron-mediated oxidation
BERENS et al. Pentoxifylline in the isolated perfused rat kidney
US5994346A (en) Use of exochelins in the preservation of organs for transplant
Chaudhuri et al. Effect of infection with M. tuberculosis and of tuberculin shock on the succinic dehydrogenase activity of guinea pig tissues
Nydegger et al. New concepts in organ preservation
Bosco et al. Use of oxygen radical scavengers on autografted pig kidneys after warm ischemia and 48-hour perfusion preservation
CA2095606A1 (en) Hydroxamic acids for preventing reperfusion injury
MXPA96004499A (en) Chlorate forming agent of novedous iron, as inhibitor of hid mediated oxidation
Elgebaly et al. Cyclocreatine inhibits the production of neutrophil chemotactic factors from isolated hearts.
MXPA99007225A (en) Method for the treatment of atherosclerosis and vascular injury by prevention of vascular smooth muscle cell proliferation
CZ278499A3 (en) Use of deferriexochelin for preparing medicament capable of preventing proliferation of vascular smooth musculature cells
US10165772B2 (en) Methods and compounds for increasing red blood cell survival
Rao et al. Effects of metabolic stimulation on cardiac allograft recovery
Bornstein et al. Potentiation of insulin action in normal subjects by a pituitary polypeptide
Hewett et al. Extraction of ACTH from human pituitaries
Simpson More humane way with seals
Kirpatovskii et al. Use of α-tocopherol emulsion for antioxidant protection of ischemic or stored kidneys

Legal Events

Date Code Title Description
EEER Examination request
MKLA Lapsed