CA2156924A1 - Water soluble non-immunogenic polyamide cross-linking agents - Google Patents

Water soluble non-immunogenic polyamide cross-linking agents

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CA2156924A1
CA2156924A1 CA 2156924 CA2156924A CA2156924A1 CA 2156924 A1 CA2156924 A1 CA 2156924A1 CA 2156924 CA2156924 CA 2156924 CA 2156924 A CA2156924 A CA 2156924A CA 2156924 A1 CA2156924 A1 CA 2156924A1
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polyamide
group
soluble
water
product
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French (fr)
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Ton That Hai
Deanna J. Nelson
David Eugene Pereira
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Baxter International Inc
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Individual
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    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08GMACROMOLECULAR COMPOUNDS OBTAINED OTHERWISE THAN BY REACTIONS ONLY INVOLVING UNSATURATED CARBON-TO-CARBON BONDS
    • C08G69/00Macromolecular compounds obtained by reactions forming a carboxylic amide link in the main chain of the macromolecule
    • 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
    • C08F8/30Introducing nitrogen atoms or nitrogen-containing groups

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  • Chemical & Material Sciences (AREA)
  • Health & Medical Sciences (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Medicinal Chemistry (AREA)
  • Polymers & Plastics (AREA)
  • Organic Chemistry (AREA)
  • General Chemical & Material Sciences (AREA)
  • Polyamides (AREA)
  • Medicinal Preparation (AREA)

Abstract

The present invention relates to water-soluble nonimmunogenic polyamide cross-linking agents and their use to cross-link, polymerize, decorate, and conjugate proteins, polynucleotides and other biological substrates to form substantially nonimmunogenic water-soluble products. The present invention also relates to proteins, polynucleotides and other biological substrates which are cross-linked, conjugated, polymerized or decorated with water-soluble polyamides to form substantially nonimmunogenic products.

Description

WO95/17886~ S 6 ~ ~ PCT~S94/14821 WATER SOLUBLE NON-IMMUNOGENIC POLYAMIDE

CROSS REFERENCE TO RELATED APPLICATION
This is a continuation-in-part of copending U.S.
patent application number 7/981,447, filed ll-25-92.
Field of the Invention The present invention relates to water-soluble, substantially non;mml7~ogenic polyamide cross-linking agents. The present invention also relates to covalent binding of water-soluble polyamides to proteins, polynucleotides and other biological substrates to form substantially nonimmunogenic water-soluble products. The present invention also relates to proteins, polynucleotides and other biological substrates which are cross-linked, conjugated, polymerized or decorated with water-soluble polyamides to form substantially non;mmllnogenic products.

Backaround of the Invention Cross-linking reagents are used for a variety of purposes, including the investigation of the spatial arrangement and functions of various macromolecular entities, the identification of binding sites (receptors) for ligands, the preparation of affinity matrices, and the modification and stabilization of diverse macromolecular structures (Methods in Enzymology, Volume 9l, pages 580 to 609 (1983)).
Cross-linkers have been designed to preserve electrostatic charge; to alter electrostatic charge;
to decrease immunogenicity; to increase and decrease susceptibility to proteolysis; to introduce fluorescent labels, spin labels, radiolabels, and electron-dense substituents; to attach several WO9S/17886 2 ~ Z ~ - 2 - PCT~S94/14821 -different types of carbohydrate moieties; to modify enzyme specificity; and to introduce intramolecular and/or intermolecular cross-links, both to couple already associated species and to join various proteins in order to combine the properties of both into a single molecule (G. E. Means and R. E. Feeney, Bioconjugate Chemistry, Volume l, page 2 to 12 (l990)). A large number of cross-linking reagents have been developed to serve these and a variety of other purposes. Many of these reagents are commercially available.
Cross-linking of proteins and their immobilization, either by attachment to an insoluble support or by various other means, has been employed to increase the stability of proteins or of certain conformational relationships in proteins; to couple two or more different proteins; to identify or characterize the nature and extent of certain protein-protein interactions or to determine distances between reactive groups in or between protein subunits.
Proteins may be immobilized to facilitate their use and their separation from other products. Cross-linking therapeutic proteins or polypeptides has been shown to decrease immunogenicity and to increase the lifetime of the cross-linked product in the blood stream.
In general, cross-linking agents consist of an organic bridge between activated termini. The termini bind to biological macromolecules to form a link.
Various organic bridges are recognized in the art, including peptides, carbohydrates (e.g., dextran, starch, and hydroxyethylstarch), fatty acids, polyglycolides, polypeptides (e.g., gelatin or collagen), polyalkylene units, and polymers such as poly(vinylalcohol), polyvinylpyrrolidone, and polyethylene glycol (also known as polyoxyethylene).

WO9Y17886 2 1 5 6 9 2 4 PCT~S94/14821 Commercially available homobifunctional and heterbifunctional cross-linking agents range in size from about 6 to 16 A. Their solubility in water decreases with chain length. Yet the efficiency of 5 cross-linking is increased with chain length as steric hindrance is reduced.
Peptides composed of three to nine amino acid residues are commonly used as cross-linking agents.
However, these suffer from the following disadvantages: the chemistries used in peptide synthesis are complex, involving selective blocking and deblocking of functional groups and specific coupling conditions. Care must be taken not to racemize the amino acid components. Peptides must be chosen carefully so that they have no biological activity. Finally, they are subject to enzymatic hydrolysis, which limits their period of utility, particularly during circulation in vivo.
Synthetic polymers are being developed for use as cross-linking agents. A synthetic polymer cross-linker desirably has the following characteristics:
(l) The polymer must be water-soluble and exhibit a narrow, definite molecular weight distribution. (2) It should provide attachment/release sites or the possibility of the incorporation of such sites. (3) The polymer should be compatible with the biological environmental, i.e., non-toxic, non-antigenic, and not provocative in any other respect. (4) It should be biodegradable or eliminated from the organism after having fulfilled its function (Duncan and Kopecek, Advances in Polymer Science, Volume 97, pages 53 to l~l (19~34)~.
The conjugation of biologically active polypeptides with water-soluble polymers such as PEG
is well-known. The coupling of biologically active and pharmaceutically active peptides and polypeptides WO95117886 2~ ~9~ ~ PCT~S94114821 -to PEG and similar water-soluble polvmers is disclosed by U.S. Patent No. 4,179,377 to Davis et al.
Polypeptides modified with PEG are disclosed as exhibiting dramatically reduced immunogenicity and antigenicity. The PEG conjugates also exhibit a wide range of solubilities and low toxicity, and have been shown to remain in the bloodstream considerably longer than the corresponding native compounds yet are readily excreted. The PEG conjugates have also been shown not to interfere with enzymatic activity in the bloodstream or the conformation of the polypeptides conjugated thereto. Accordingly, a number of PEG-conjugates of therapeutic proteins have been developed exhibiting reduced immunogenicity and antigenicity and longer clearance times, while retaining a substantial portion of the protein's physiological activity.
Attention has also focused upon the conjugation of PEG with therapeutic drugs. Gnanov et al., "Macromolecules," 17, pages 945 to 952 (1984) observed that the attachment of PEG to various drugs led to prolonged pharmacological activity.
U.S. Patent No. 5,122,614 to Zalipsky describes the use of polyethylene gycol as a cross-linking agent. U.S. Patent No. 5,053,520 to Bieniarz describes polyamino acid based coupling agents which are not water-soluble. U.S. Patent No. 4,182,695 to Horn describes protein bound to polyamides. Russian Patent Application No. SU 1659433 discloses water-soluble polyamides with luminescent groups in the 30 chain. U.S. Patent No. 5,110,909 to Dellacherie discloses water-soluble macromolecular conjugates of hemoglobin. PCT Application WO 92/08790 to Cargill discloses the use of polyamide polymers bonded to a linker group which is bonded to a protein.
Many potentially therapeutic proteins have undesirable characteristics such as short half life in 2~92~
WO95117886 PCT~S94/14821 vivo, poor solubility, vulnerability to enzymatic degradation in vivo, or immunogenicity. The polyamides of the present invention when coupled to such proteins overcome these disadvantages.

Summarv of the Invention The present invention is water-soluble, substantially non;mml1nogenic polyamides having number average molecular weights of about 300 to about 20,000 grams per mole; where the amide repeat units are comprised of: (i) a water-soluble organic acid subunit having at least one carboxylate group and fifteen or fewer atoms separating the amide functionalities in the polyamide; covalently linked as an amide to (ii) a water-soluble organic amine subunit having at least one primary amino group and fifteen or fewer atoms separating the amide functionalities in the polyamide.
In other words, the polyamide of the present invention is a water-soluble, substantially non;mml~nogenic polyamide selected rom the formulas I, II, and III:
I Y-A-X-Y
II Z-B-X-Z
III Y-X-Z
(i) where terminus Y is OH or a carboxyl coupling group; (ii) where terminus Z is H or a coupling group attached to an amine group; and (iii) where X is a polyamide selected from: (B-A)n, (A-B)n, (B-A')n or (A'-B)n and branched polyamides formed by linking (B-A)n, (A-B)n (B-A')n or (A'-B)n to a central polyacid, polyamine or polyamino acidi and (iv) where A is a ~,~-di-acid; B is a ~,~-diamine; A' is a ~,~-amino acid having the formula YlOC-CH2-CH-S-(CH2)m-Xl-CH2-CH2-X2-(CH2)m-S-CHCH2-COY

WO9S/17886 2 ~ 6 - PCT~S94/14821 -where Y1 has the formula - OC-(CH2)p-NH-where p is from 1 to about 4, m is from about 2 to about 4, X1 and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N, and R3 is a lower alkyl having from about 1 to about 2 carbon atoms; n is the number of amide repeat units in the polyamide; and (v) where the acid subunits of the amide repeat units are (a) organic acids having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N present as substituents on or atoms in the chain, or (b) two or more of such organic acids bridged by water-soluble organic diamines; and (vi) where the amine subunits of the amide repeat units are organic, water-soluble amines having at least one primary amine group and having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N present as substituents on or atoms in the chain; and (vii) where n is from 2 to about 100.
The present invention includes one or more such polyamides used to cross-link, conjugate, decorate or polymerize proteins, antibodies, haptens, polypeptides, polynucleotides or other biological substrates. The cross-linked, conjugated, polymerized or decorated product is water-soluble, substantially non;mmnnogenic and retains all or a useful portion of the physiological activity of the substrate.

WO95/17886 21 5 6 ~ 2~ PCT~S94114821 Brief 3escri~tisn of the Drawinas Figure 1 shows the polycondensation of ethylene glycol bis(methoxycarbonylmethyl ether) and 1,4-diaminobutane.
Figure 2 shows the reaction conditions, product characteristics, and yield of the reactions shown in Figure 1.
Figure 3 shows the experimental data, including oxygen binding function of diaspirin cross-linked hemoglobin polymerized and decorated with PAS-2400.
Figure 4 shows the size exclusion chromatographic profiles of diaspirin cross-linked hemoglobin polymerized and decorated with PAS-2400.
Figure 5 shows the reverse phase HPLC profiles of diaspirin cross-linked hemoglobin polymerized and decorated with PAS-2400.
Figure 6 depicts the components of polyamide synthesis.
Figure 7 depicts the synthesis of BMDAB (a polyamide component).
Figure 8 depicts the polycondensation of BMDAB
with diamine, to form a polyamide.
Figure 9 depicts the synthesis of polyamide activated esters PAS-3037 and PAS-4200.
Figure 10 depicts the synthesis of maleimide-capped polyamide, designated PAM-4080.
Figure 11 depicts the size exclusion profiles following polymerization of diaspirin cross-linked hemoglobin with PAS-3037.
Figure 12 depicts size exclusion chromatography - following polymerization of diaspirin cross-linked hemoglobin with PAS-4200.
- Figure 13 depicts the reverse phase HPLC
profiles following polymerization of diaspirin cross-linked hemoglobin with PAS-4200.

WO95/17886 1 ~ ~9 ~1 PCT~S94/14821 -Figure 14 depicts the size exclusion chromatography profiles following polymerization of diaspirin cross-linked hemoglobin with PAM-4080.
Figure 15 depicts reverse phase HPLC following polymerization of diaspirin cross-linked hemoglobin with PAM-4080.
Figure 16 shows the experimental data foIlowing polymerization of diaspirin cross-linked hemoglobin with PAS-3070.
Figure 17 shows the experimental data following polymerization of diaspirin cross-linked hemoglobin with PAS-4080.
Figure 18 shows the experimental data following polymerization of diaspirin cross-linked hemoglobin with PAM-4080.

Detailed Descri~tion of the Invention The polyamides of the present invention are substantially non-immunogenic, water-soluble polyamides having number average molecular weights of about 300 to about 20,000 grams per mole. The amide repeat units of these polyamides are composed of a water-soluble organic acid subunit having at least one carboxylate group and fifteen or fewer atoms separating the amide functionalities in the polymer, covalently linked as an amide to a water-soluble organic amine subunit having at least one primary amino group and fifteen or fewer atoms separating the amide functionalities in the polymer. These polyamides may be employed directly or after activation, for the purposes of cross-linking, conjugating, polymerizing and/or decorating biological substrates such as proteins, polypeptides, antibodies, haptens, carbohydrates or polynucleotides to give products which are water-soluble, substantially non1mm~]nogenic, and which retain all or a useful ~ WO95/17886 2 ~ ~ ~ 9 2 ~1 PCT~S94/14821 _ g _ portion of the substrate's physiological activity.
They may also be used to attach substrates to detection agents or solid matrices.
The term "substantially non-immunogenic"
S indicates that the polyamide does not elicit a humoral or cell-mediated immune response, either in vivo or in vitro.
The term "water-soluble" indicates that the polyamide has a solubility in water that exceeds 500 mg per 100 mL. The term also indicates that the polyamide does not act as a detergent and does not form aggregates such as micelles in water.
The term "activation" means converting a group located on a polyamide terminus to a more reactive coupling group.
The polyamide may be linear or branched.
The term "substrate" means the molecule to which the polyamide of the present invention is bound.
Substrates include but are not limited to proteins such as enzymes, growth factors, antibodies or blood proteins; polynucleotides such as complementary DNA
fragments; steroids and hormones; immunoconjugates;
carbohydrates; and conjugates of any of these substrates. The substrate may also be a solid support or bead. Substrates include molecules having therapeutically useful biological activity.
As used herein, a substrate is said to be "decorated" when multiple polyamides are bound to the substrate by one terminus of each polyamide and all other termini of the polyamide are not bound to a different substrate molecule.
The water-soluble polyamides of this invention may be prepared by methods known in the art. Known methods for the preparation of polyamides are incorporated here by reference as useful methods for the preparation of the polyamides of the present WO95/17886 PCT~S94/14821 -2~ 24 - 10 -invention. N. Ogata et al., Polymer Journal, Volume 5, pages 186ff (1973) and N. Ogata and Y. Hosoda, Journal Polymer Science, Polymer Lett. Ed., Volume 12, pages 355ff (1974) describe the polycondensation of diesters activated by ether or hydroxyl groups with diamines. N. Ogata et al., Journal Polymer Science, Polymer Chemistry Ed., Volume 14, pages 783ff (1976), N. Ogata et al., Polymer Journal, Volume 11, pages 827 to 833 (1979), and H. Sato, et al., Makromol Chemistry, Volume 182, page 755 to 762 (1981) describe the polycondensation of activated diesters containing ether, thioether or hydroxyl groups with diamines. D.
Kieley and T-H. Lin have also described polyhydroxypolyamides and a process for making same, U.S. Patent No. 4,833,230. N. Ogata and Y. Hosoda, Journal Polymer Science, Polymer Chemistry Ed., Volume 18, pages 1159 to 1162 (1978) describe the synthesis of water-soluble polyamides by polycondensation in solutions of ethylene glycol dimethoxycarbonylmethyl ether and hexamethylene diamine.
The acid subunits of the amide repeat units are selected from the group of organic acids having fifteen or fewer atoms in the chain and having heteroatoms (O, S, P, N) present either as substituents on or atoms in the chain. Alternatively, the acid subunits of the amide repeat units may consist of two or more such organic acids joined to bridging water-soluble, organic diamines. The amine subunits of the amide repeat units are selected from among the group of organic amines having fifteen or fewer atoms in the chain and having heteroatoms (O, S, P, N) present as substituents on or atoms in the chain. Polyamides of similar and/or dissimilar structure may be linked by a central polyacid, polyamine or polyamino acid to form branched, water-soluble polyamides.

21~692~
WO95/17886 PCT~S94/14821 In one embodiment of the present invention, X is a polyamide selected from (B-A) n~ (A-B) n~ and branched ~ polyamides formed by linking (B-A) n or (A-B) n to a central polyacid, polyamine or poly(amino acid). In this embodiment, the acid subunits of the polyamide repeat units are two or more organic acids each of said organic acids having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O other than carboxyl or carbonyl 0, S, P or tertiary N present as substituents on or atoms in the chain bridged by a water-soluble diamine having the formula -NH-Rl-NH- where Rl is a substituted or unsubstituted aliphatic chain having from about 4 to about 5 carbon atoms. In a preferred embodiment of the present invention, the water-soluble diamine having the formula -NH-Rl-NH- is l,4-diaminobutane.
In another embodiment of the present invention where X is a branched or unbranched polyamide selected from (B-A) n or (A-B~ n~ the acid subunits o~ the amide repeat units are organic acids having the formula -OC-CH-CH2-S-(CH2)m-Xl-CH2-CH2-X2-(CH2)m-S-CH2CH-CO-where m is from about 2 to about 4, Xl and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N, and R2 is H or acetamide. In these polyamides, the sulfur group is located in a position ~ to each of the terminal carboxyl groups. In a preferred embodiment of the present invention, Xl and X2 are both 0. In a more preferred embodiment of the present invention, Xl and X2 are both O and m is 2.
Compounds in accordance with this aspect of the present invention have several advantageous features when used with substrates having therapeutic WO95/17886 ~ 2 ~ PCT~S94/14821 -biological activity. These compounds are less reactive which permits greater control following activation to m; n i mi ze hydrolysis. This, in turn, optimizes coupling with protein substrates. These polyamides are also effective oxygen radical quenchers.
In yet another embodiment of the present invention when X is a branched or unbranched polyamide having the formula (B-A')n or (A'-B)n, the acid subunits of the amide repeat units are organic acids having the formula Yloc-cH2-cH-s-(cH2)m-xl-cH2-cH2-x2-(cH2)m-s-cHcH

where Yl has the formula - OC-(CH2)p-NH-where p is from l to about 4, m is from about 2 to about 4, Xl and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N, and R3 is a lower alkyl having from about l to about 2 carbon atoms. In a preferred embodiment of the present invention, Xl and X2 are both O. In a more preferred embodiment of the present invention, Xl and X2 are both O, m is 2, and R3 is methyl.
In accordance with the present invention, A' is an a, ~-di-acid having the formula Yl-A-Yl, where Y
has the formula -OC(CH2)p-NH- where A is an a, ~-di-acid as described herein above.
Any of the known coupling chemistries may be used to activate polyamides of this invention to decorate, link, polymerize and/or conjugate substrates. Many examples of such coupling chemistries are given in "Chemistry of Protein Conjugation and Cross-linking," ~. Wong, CRC Press, Inc. (l99l) which is incorporated by reference herein.

21~6924 WO95117886 ' PCT~S94114821 Such chemistries include reacting the polyamides with bi- or poly- functional protein reagents such as ~ dialdehydes, N-hydroxysuccinimide esters, functionalized acetals, bis-maleimides, bifunctional imino esters, diepoxides, and dicarboxylic acid chlorides. The choice of coupling chemistries will depend upon the substrate molecule being cross-linked, conjugated, polymerized and/or decorated. The coupling chemistry should be selected so that it does not alter the biological or chemical activity of the substrate molecule.
Generally, to decorate a substrate molecule, between about 4 and 50 moles of polyamide should be used per mole of substrate. Larger substrate molecules will require a greater proportion of polyamide. To primarily conjugate, cross-link or polymerize a substrate without decorating requires the knowledge of a chemist skilled in the art as to the chemistries of the coupling agents, the reactive groups on the particular substrate, the size of the substrate, the size of the polyamide, concentration of the substrate, and general reaction parameters.
As will be appreciated readily by those of skill in the art, substrates such as amino acids, peptides, proteins, nucleotides, polynucleotides, pharmaceutic agents, and diagnostic agents have functional groups which may be covalently bound to the pendant functional groups of the polyamide backbone and functionalized derivatives thereof. Those of ordinary skill in the art having the benefit of this disclosure will comprehend the synthetic approaches that may be employed to covalently join the polyamide and the substrate. The order of reaction is not important.
The pendant functional group(s~ of the polyamide may be activated appropriately, if so required, and then attached to the substrate. Likewise, the substrate WO95/17886 2 ~ ~ G g ~ 4 PCT~S94/14821 -may be activated appropriately, if necessary, and then attached to the polyamide.
For example, amino, hydroxy, carbonyl, carboxyl, or thiol substituents are commonly found as part of the structure of amino acid, peptide, protein, nucleotide, polynucleotide, and diagnostic agent compounds. Moreover, the polyamide may be synthesized to incorporate reactive termini such as these substituents. The substrate may be joined to the polyamide by chemistries such as those cited below, or by other chemistries such as those disclosed in Bodanszky and Bodanszky, "The Practice of Peptide Synthesis," Springer-Verlag, New York, (1984);
Lundblad, "Chemical Reagents for Protein Modification," CRC Press, Boca Raton, Florida, (l99l);
Mosbach "Methods in Enzymology, Volume XLIV, Immobilized Enzymes," Academic Press, New York, (1976); or U~lm~nn and Peyman, "Antisense Oligonucleotides: A New Therapeutic Principle,"
Chemical Reviews, Volume 90, No. 4, pages 543 to 585 (June l990).
For example, biotin is recognized as a diagnostic probe that is selectively retained by complexation with avidin. Biotin contains a carboxyl group that may be activated as a succinimidyl ester and attached to a polyamide having a amino terminus.
Either prior to or following covalent bonding to biotin, the other terminus of the polyamide may be covalently bonded to a peptide, protein or other biochemical agent. Under these conditions, the polyamide serves as a spacer group that concurrently maintains or increases the aqueous solubility of the product. The biochemical agent is thereby labeled with a diagnostic probe that is positioned at the end of the polyamide spacer to facilitate interaction with avidin.

21~6~24 WO95/17886 PCT~S94/14821 Similarly, deferoxamine is a pharmaceutic agent that is used therapeutically as an antidote to iron ~ poisoning. The duration of therapeutic action of deferoxamine is short, because it is rapidly excreted via the kidney. It has been recognized that if deferoxamine is conjugated to a larger molecular weight entity such as a dextran or albumin, it will be retained in the vascular circulation for longer periods of time. In accordance with the present invention, a polyamide may be used as a spacer group that concurrently maintains or increases the aqueous solubility of the product. One terminus of the polyamide may be converted to a carbonyl functional group and attached to the amino substituent of deferoxamine by reductive amination, and the other terminus of the polyamide may be converted to an activated ester (e.g. a succinimidyl ester) and attached to albumin. Through this conjugation, the duration of vascular circulation of conjugated de~eroxamine is lengthened and the agent retains its chelating abilities.
All the components of the polyamides of the present invention are selected so as to preserve water-solubility. They are water-soluble, hydrophilic over the entire chain length. The length o~ the polyamide is chosen to facilitate interaction between the substrate and the polyamide. The cross-linking of a large substrate will require a longer polyamide since it will minimi ze steric interactions between two large substrate molecules.
An immunogenic substrate should generally be highly decorated and should have relatively long chain polyamides.
In reacting the polyamides of the present invention to biologically active substrates, such as enzymes, care is taken to avoid destroying the WOgS/17886 2 ~ ~ ~ 92~:; PCT~S94/14821 ~

activity of the substrate. One skilled in the art will understand that varying the degree of decoration and/or polymerization will allow one to prepare a product having a useful biological activity.
The polyamides of the present invention are not polymers of a-amino acids, so they are not subject to enzymatic hydrolysis.
In addition, the polyamides of the present invention may be used to render substrates soluble in organic solvents such as methanol, ethanol or acetonitryl.
The polyamides of the present invention may be used as polymerization agents. In one example described fully below, the t~rm;n; of a polyamide have been modified as maleimide groups, suitable for reaction with thiol substituents of proteins.
Bis(maleimide) polyamide was employed to polymerize human hemoglobin via the cysteine-~93 thiol residues of that protein. Similarly, in another example below, the t~rm;ni of a polyamide were converted to bis(succinimidyl) esters or bisaldehydes, suitable for reaction with amino substituents of proteins. Both the bis(succinimidyl) polyamide and the bisaldehyde polyamide have been employed to polymerize human hemoglobin via the a-aminO groups of lysine residues of the protein.
In another embodiment the polyamides of the present invention may be used to link probes (e.g., fluorescent, radioactive, etc.) to a substrate to be detected.
In the examples that follow, we use the following nomenclature for our polyamides: since the backbone is a polyamide, the letters PA will apply;
the letter designating the coupling group will follow, M for maleimide and S for N-hydroxysuccinimide; a hyphen will separate the alphabetic code from the 21~92~
WO95/17886 PCT~S94/14821 approximate molecular weight. In a preferred embodiment of the present invention the polyamide is ~ bis(maleimidoacyl) polyamide. In a more preferred embodiment of the present invention the polyamide is bis(maleimidoglycyl) polyamide. Thus, a polyamide identified as PAM-3800 is a polyamide bis(maleimide) having a molecular weight of about 3800 Daltons.

DESIGN AND SYNTHESIS OF POLYAMIDES
10In the following examples the polyamide condensation products are characterized in three ways.
Size exclusion chromatographic (SEC) analysis is completed using a SuperoseTM 12 column and 50 mM
phosphate, pH 6.5, mobile phase delivered at a flow rate of 0.~ mL~min. with detection at 220 nm; this analysis confirms that polymerized products were formed and permits approximation of molecular weights and the range of molecular weights of the components in the product mixture. Thin-layer chromatographic (TLC) analysis permits separation and characterization of end-group functionality of the components in the product mixture. The structure of each component is assigned on the basis of relative migration (Rf) and reactivity toward ninhydrin spray reagent. Under the TLC conditions, polyamides with diester end-groups have the largest Rf, followed by components with mono-ester/mono-amine end-groups, and di-amine end-groups, respectively. Only components having an amine end-group are reactive toward ninhydrin. The structure of the mono- and di-esters is confirmed by base-catalyzed hydrolysis and TLC of the resulting products; under these conditions esters are hydrolyzed to acids and the Rf of the material decreases. Finally, the molecular weight is estimated by amino end-group analysis using fluorescamine. Precisely and accurately weighed polyamide samples are dissolved in 2 ~
WO95/17886 ~ ' PCT~S94/14821 -methanol/phosphate buffer, derivatized by adding fluorescamine dissolved in acetone, and then analyzed by flow injection with a HPLC system equipped with a fluorescence detector. Equivalent weights are determined by comparison of responses for standard solutions of diaminohexane/PEG/ethyl acetate in methanol/phosphate buffer. Equivalent weights are converted to number average molecular weights based on the average number of amines per molecule.
Alternatively, the NMR spectrum can be used to estimate the number average molecular weights of the polyamides, as follows: the first step is to divide the structure of the polyamide into end groups and repeating units. Then the molecular weight of each part is calculated. Next one identifies unique components in each part and correlates the corresponding NMR resonance with that component.
Polyamides have a number of well-resolved resonances that can be correlated with specific functional groups. For example, the two pairs of two hydrogens on the succinate group in PAS-4200 give rise to (triplet) resonances at about 2.53 and 2.92 ppm having integrals of 2.197 and 2.605 units, respectively.
Similarly, the internal methylene groups of the butanediamine residue give rise to a broad resonance at 1.5 ppm having an integrated area of 16.034 units.
There are two succinate residues in the end groups of the polyamide derivative: therefore, the resonance at about 2.53 ppm and the one at 2.92 ppm each results from four hydrogens. The average area response is ~2.197 + 2.605)/2 or 2.401 units per four hydrogens on each succinate. Similarly, the two internal methylene groups of the butanediamine residue in the repeating unit contain four hydrogens. The observation that the integrated area of the latter resonance (16.034 units) is larger than that of the ~ WO95/17886 2 ~ ~ 6 9 ~ 4 PCT~S94/14821 four-hydrogen response for either type of succinate hydrogen indicates that there are multiple ~ butanediamine residues within the repeat units in the polymer. We can estimate the value of the multiple by ~ 5 ratioing the integrated areas: 16.034/2.401 or approximately 7. Thus, there are seven repeat groups in the polyamide. The molecular weight of the polyamide is the sum of the molecular weights of each of the end groups (416.44 and 198.14, respectively) and the multiple seven times the molecular weight of the repeat unit (7 x 504.57 or 3532). The sum is 4146.57 or about 4200 Da. This value was also obtained independently by end-group analysis of the polyamide bisamine precursor of PAS-4200 using fluorescamine.

SYnthesis of PAS-2400 ~xam~le l(a) PolYcondensation of Ethvlene ~1YCO1 bis(methoxycarbonvlmethvl) and 1,4-diaminobutane.
Ethylene glycol bis(methoxycarbonylmethyl) ether (EDE), which has an ether group as a substituent ~ to each ester group, was condensed with 1,4-diaminobutane (DAB) to produce polyamides. See Figure 1. Two poly-condensation methods were used: the solution methodand the melt method.
In general, the polycondensations were completed as follows. For the solution method, EDE and DAB in the desired molar ratio were dissolved in methanol, and the solution was heated at 30C for seventy two hours or at 65C for twenty four hours. The solvent was evaporated and the residue was treated with acetone and repeatedly evaporated to remove residual methanol. Trituration of the residue with acetone afforded a solid. In the melt method, a mixture of EDE and DAB was heated at 120C under vacuum with W O 95/17886 - PCTrUS94114821 magnetic stirring to remove methanol. After one to two hours the mixture was dissolved in methanol. The solution was evaporated to dryness and the residue was triturated with acetone to give polyamide product.
Analysis of the reaction mixtures by SEC
confirmed that polymerized products were formed. TLC
analysis (stationary phase: silica gel; eluent: 2-propanol / NH40H / H20, 7:1:2, by volume) of the product showed three spots having Rf values of 0.1, 0.4, and 0.7, respectively. The structures of the corresponding polyamides were assigned on the basis of reactivity toward ninhydrin and base as a, ~-diaminopolyamide (designated I in the figure), ~-amino-~-esterpolyamide (designated II), and ~,~-diesterpolyamide (designated III), respectively(Figure 1). In addition, product III is ninhydrin-negative while products I and II are ninhydrin-positive, indicating the products has at least one primary amine group. Finally, products II and III can be hydrolyzed with dilute aqueous NaOH, whereas I
cannot, indicating products II and III contain at least one ester group.
The yield of these products depends on the molar ratio of DAB to EDE. A molar ratio of one gives I as the major product. A molar ratio of DAB/EDE greater than one gives polyamide II as the major product. In contrast, III became the major product with a molar ratio of DAB/EDE of less than one. The results of polycondensation of EDE and DAB are summarized in Figure 2. The experimental data indicate that ~-amino-~-ester polyamide II having a number average molecular weight (MW) of about 2,400 Dalton is best produced by the solution method at 30C. ~,~-Diamino-polyamide I having a MW in the range of 1,300 to 1,500 Dalton could be prepared either by the solution or the melt method employing a DAB/EDE molar WO95/17886 2 15 6 9 2`4 . PCT~S94114821 ratio of l.3 to l.5. ~,~-Diester-polyamides III were obtained in good yield by the melt method with equimolar EDE and DAB. Because DAB is a volatile compound, DAB is gradually removed from the reaction mixture when the melt method is utilized, leaving EDE
in large excess. Conseauently III is obtained as the major product.

Exam~le l(b) Conversion of ~olyamide III to an activated cross-linkina aaent.
Crude diester III (Figure l), obtained by condensation of EDE and DAB, was hydrolyzed with dilute sodium hydroxide to the corresponding di-acid.
After hydrolysis, the reaction mixture was treated with AG50W-X8 resin (BioRad) to remove sodium ion and by-products I and II. The di-acid was obtained in a pure state as judged by TLC. The di-acid was treated with dicyclohexylcarbodiimide (DCC) and N-hydroxysuccinimide (NHS) in chloroform to convert it to the corresponding polyamide bis(N-hydroxysuccinimide ester) (designated PAS-2400).

Exam~le 2 PolYmerization of Hemoalobin with PAS-2400.
A typical polymerization of diaspirin cross-linked hemoglobin (designated DCLHb) with PAS-2400 was completed as follows. DCLHb was prepared according to the method described in U.S. Patent No. 5,128,452. A
solution of DCLHb in O.l M HEPES of about pH 7 to 8 was deoxygenated by successive vacuum / nitrogen cycles for one and a half hours at room temperature.
PAS-2400 was dissolved in deoxygenated water, and the solution was added immediately to the DCLHb solution.
The reaction mixture was stirred at room temperature under nitrogen, and the reaction was monitored by size ~ ~ } ~ ~ i WO95/17886 2 ~ 2 4 PCT~S94/14821 -exclusion chromatography using TSK-G4000SW brand and TSK-G3000SW brand columns connected in series with mobile phase consisting of 2-propranol/50mM phosphate buffer, pH 6.5 (l:9, v/v), delivered at a flow rate of l mL/minute detection at 280 nm. The latter method demonstrated that the polymerization was completed in less than thirty minutes and that polymerization was accompanied by decoration. The solution was cooled to 5C and a solution of l M NAC (N-acetyl-L-cysteine) (molar ratio of NAC/Hb about 5:l) was added. The solution was stirred at 5C under nitrogen overnight and then dialyzed against lactated Ringer's solution to give the final product. Experimental data are summarized in Figures 3, 4, and 5. Note: In the figures NHS-PA 6 is an alternate designation for PAS-2400.
The data indicate the following. The yield of oligomer is increased with increasing ratios of PAS-2400 to DCLHb. SEC elution times of DCLHb monomer decrease with increasing molar ratios of PAS-2400, indicating that PAS-2400 decorates DCLHb.
Polymerization is fast; it was complete in less than thirty minutes. However, competitive hydrolysis of the polymerization agent is also fast. As the solution pH is increased, higher yields of high molecular weight polymers are obtained. For example, five eguivalents of PAS-2400 give 7%, 17%, and gel, respectively, of high molecular weight polymers at values of pH of 7.0, 7.5, and 8.0, respectively.
P50 values and n values of DCLHb polymerized with PAS-2400 are in the range of 29 to 33 mm Hg and l.8 to 2.l, respectively. P50 is the oxygen partial pressure at which hemoglobin is half saturated while the "n" value is a measure of the cooperativity of oxygen binding. The Pso of human hemoglobin in red blood cells is about 28. Thus, the excellent oxygen-WO95/17886 ~ 1 5 6 9 2 4 PCT~S94/14821 binding function of DCLHb is maintained in thesepolymers. RP-HPLC analysis (Figure 5) indicates than ~ both a~ - and ~-chains are modified. However, ~-chains apparently are more extensively modified than are ~-ch~;n~.
Thus, PAS-2400 can be used to produce decorated, polymerized DCLHb. The short reaction time (thirty minutes) is favorable for large-scale synthesis. Two to four equivalents of PAS-2400 at pH 7.0 are suitable for polymerization. The hemoglobin maintains its biological activity, i.e., oxygen binding and, as described below is nonimml7nogenic.

Exam~le 3 Methods for the Synthesis of Lonaer PolYamides.
Longer polyamides are obtained if the lengths of the component acid and amine are increased, i.e., polymerization with adipic acid (six carbons) or 1,6-hexanediamine (six carbons) yields longer polymers than does polymerization with succinic acid (four carbons) or 1,4-butanediamine (four carbons). However, increases in chain length using hydrocarbon components would reduce the aqueous solubility of the protein.
With this in mind, we synthesized polyamides from diester EDE and each of two longer diamines:
ethylene glycol bis(3-aminopropyl) ether (EGBE; MW
176) and diethylene glycol bis(3-aminopropyl) ether (DGBE; MW 220). See Figure 6. The SEC retention times of each of the polyamides suggested these products had higher molecular weights, but the products were waxy and had low melting points.
Purification of such products by crystallization is extremely difficult.
To mi n i mi ze these shortcomings we combined three concepts to select appropriate activated esters for the synthesis of longer polyamides. First, we WO95/17886 2 ~ 5 ~ 3 2 ~1 PCT~S94ti4821 ~

identified components that are di-acids having ~-ether links; these di-acids are easily converted to activated diesters. Our initial di-acid of choice was diglycolic acid. Second, we converted one end of this di-acid to an amide by reacting two equivalents of di-acid with one equivalent of diamine; this generated a new and longer di-acid that we can use as a component for longer polyamides. Our first di-acid of choice was 1,4-(carboxymethoxyacetamido) butane, which we used as the activated methyl diester BMDAB (MW 348).
Insertion of the methylene (hydrocarbon) groups reduced the flexibility of the molecule sufficiently to render it a crystalline solid and retention of the ether link preserved the solubility in water. Third, we increased the length of the diamine component in a way that will maintain water solubility; thus, we used ethylene glycol bis(3-aminopropyl) ether (EGBE) and diethylene glycol bis(3-aminopropyl) ether (DGBE) as the diamine components in polyamide synthesis.
The activated diester building block, BMDAB, was obtained in two steps (Figure 7). DAB (1,4-diaminobu-tane) was allowed to react with two equivalents of glycolic anhydride in N,N-dimethylformamide (DMF) to give an almost quantitative yield of BCDAB [1,4-bis(carboxymethoxyacetamido) butane]. The latter was esterified in methanol in the presence of aqueous HCl or HCl in dioxane solution. The advantage of using HCl in solution is the ease of carrying out the reaction, especially in a large scale synthesis, and the observation that an exact amount of HCl can be employed to avoid the formation of by-products.
Gaseous HCl was tried, but a by-product was detected in the product mixture.
In contrast to the polycondensation of EDE and DAB by the solution method, which gives the ~-methylester-~-aminopolyamide as the major product ~ 56924 WO95/17886 PCT~S94/14821 when a molar ratio of EDE to DAB of 1 was used, the polycondensation of equimolar ~uantities of BMDAB and EGBE or DGBE or of molar ratios of BMDAB to DGBE of greater than 1 (Figure 8) gave mixtures containing substantial amounts of three products: an a-ester-~-amine (reactive to ninhydrin; hydrolyzed by base); an a,~-diamine (reactive to ninhydrin); and a a,~-diester (unreactive to ninhydrin). Unfortunately, thepresence of large amounts of other products made the purification of a desired product tedious. However, we found that the use of an excess of diamine (e.g., a molar ratio of diamine to BMDAB of 1.3) gave the a,~-bisamine polyamide as the major product containingonly very small amounts of the monoamine by-product.
This latter procedure is therefore preferred to produce the polyamide backbone of the polymerization reagents.

Exam~le 4 Conversion to Activated Polvmerization A~ents:
Pol~amide bis(N-hvdroxvsuccinimide) ester.
The first attempt to synthesize polyamide bis(N-hydroxysuccinimide) ester (designated PAS-3070) was a three step synthesis from BMDAB and EGBE (Figure 9).
First, EGBE and BMDAB in a molar ratio of 1.3 to 1.0 were condensed by the solution method using methanol as solvent at 65C for 24 hours to give a slightly orange solution. The product could be decolorized by adding decolorizing charcoal (NoritTM A) to the solution, filtering, and evaporating to dryness. A
white product (Figure 9, 2a), having a MW of 2700, was isolated by crystallization from methanol-acetone.
The product was not stable and turned yellow during storage. Second, conversion of the white product to the corresponding bis(2-carboxyethylcarbonyl) polyamide (Figure 9, 3a) was completed by reaction of WO95/17886 ~ S 69~4 PCT~S94114821 (2a) with succinic anhydride in DMF (a small amount of methanol was added to enhance to the solubility of 2a). The reaction produced a yellow product mixture containing bis(2-carboxyethylcarbonyl)polyamide (3a) as the major product and two minor by-products: the methyl ester of (2a) and an unknown by-product containing a free amino group as indicated by TLC.
Therefore, the mixture was treated with sodium hydroxide to convert the methyl ester to bis(2-carboxyethylcarbonyl)polyamide, (3a) and then stirredwith cation exchange resin (AG50W-X8) to absorb polyamide amine by-product. After removal of the resin by filtration, the filtrate, which contained a single product as indicated by TLC, was concentrated.
Pure product bis(2-carboxyethylcarbonyl)polyamide (3a) was obtained by crystallization from methanol/acetone.
Third, conversion of the pure product to the activated diester (4a) (designated PAS-3070) was accomplished by treatment with N-hydroxysuccinimide in the presence of dicyclohexylcarbodiimide (DCC) in DMF. The polyamide bis(succinimide ester) was soluble in water but the coupling groups were slowly hydrolyzed. Therefore when dissolved in water the activated polymerization agent was used without delay.
The synthesis described above has several drawbacks. For example, the isolated white product, (2a) is not stable; it is oxidized during storage to an unknown yellow product which could not be removed readily by crystallization. Furthermore, recrystallization of bis(2-carboxyethylcarbonyl) polyamide (3a) in methanolJacetone converts some of the di-acid to the corresponding methyl ester(s). To avoid these drawbacks, our preferred synthetic strategy is as follows. First, steps 1 and 2 (Figure 9) were carried out as an integrated process in which product 3 in Figure 9, obtained from Norit A

WO95/17886 21 5 ~ 9 2 4 PCT~S94/14821 treatment, is not isolated but is allowed to react ;mme~; ately with succinic anhydride to mask the amino ~ groups which tend to be oxidized to colored product.
Such a "one-pot" synthesis increased the yield of 3 in Figure 9, because all crude 2 is used for the second step instead of the 50-60~ of isolated product 2 that was converted in the method described above. In addition, the use of methanol as crystallization solvent for 3 was excluded to avoid the formation of methyl ester of 3.

Exam~le 5 Svnt~esis of PAS-4200.
PA5-4200 (Figure 9, 4b) was prepared using the inteqrated approach above.

~xam~le 6 Conversion to Activated Polvmerization Aqents:
Polyamide Bis(maleimido~ro~ionate).
Synthesis o~ polyamide bis(maleimidopropionate) (designated PAM-4080) was completed as a "one-pot"
two-step synthesis which is summarized in Figure lO.
Crude polyamide bisamine (Figure lO, 2B) was obtained by heating BMDAB and DGBE in refluxing methanol for 24 hours followed by decolorizing with Norit A and was immediately treated with N-hydroxysuccinimido-3-maleimidopropionate (SMP, Figure lO, 5) to give 6b.
The first attempt to carry out the latter step by mixing 2b and 5 in a molar ratio of l:2 in chloroform in the presence of triethylamine gave a higher molecular weight product. Since SMP is a bifunctional cross-linking reagent, it could polymerize 2b under these conditions. Increasing the SMP/2b molar ratio to 4.5 and the slow addition of 2b in chloroform containing triethylamine to a solution of SMP in chloroform eliminated the polymerization of 2b by SMP.

WO95/17886 2 ~ ~ g ~ 2 il PCT~S94/14821 -Thus, crude product 6b, obtained by this procedure, was mixed with cation-exchange resin (AG50W-X8) to remove unreacted polyamide amine and the purified polyamide polymerization agent 6b (designated PAM-4080) was obtained by crystallization of crude productfrom methanol/acetone. In contract to PAS
derivatives, PAM derivatives are stable in water.
Examle 7 Polvmerization of DCLHb with Polvamide Pol~merization Reaqents.
A typical polymerization of DCLHb with PAS
derivatives of the type described in Examples 4 and 5 above or PAM derivatives of the type described in Example 6 above was completed as follows. A solution of DCLHb (lO g/dL for PAS and 20 g/dL for PAM) was deoxygenated by successive vacuum/nitrogen cycles for l.5 hours at room temperature. Polyamide reagent in deoxygenated water was added immediately to the DCLHb solution. The reaction mixture was stirred at room temperature under nitrogen and the course of the reaction was followed by SEC. Polymerization was completed within 2 to 3 hours for PAS derivatives and overnight for PAM derivatives. The reaction mixture was cooled to 5C; the solution pH was adjusted to 8.0 with l molar HEPES pH 9.0 and a solution of l M N-acetyl-L-cysteine, pH 9.0 (molar ratio NAC/DCLHb of 5) was added. The solution was stirred at 5C under nitrogen overnight and then dialyzed against lactated Ringer's solution to give the ~inal product.
Experimental results are summarized in Figures ll to 18.
Polymerization of DCLHb with the activated ester PAS derivatives may be summarized as follows. (a) The degree of polymerization and the yield of oligomers increased with the molar ratio of PAS used. (b) ~¦ WO 95/17886 2 15 6 9 2 4 PCT/US94/14821 Concurrent with increases in the molar ratio of PAS
used, the elution time of DCLHb monomer decreased, suggesting that decoration of DCLHb by PAS is occurring. (c) Polymerization was fast; it was 5 complete within 2 to 3 hours. (d) The SEC profiles of polymeric product obtained by employing five equivalents of PAS-3070 and three equivalents of PAS-4200 are very similar. This also demonstrates that longer reagents facilitate polymerization of DCLHb.
(e) Four equivalents of PAS-3070 and 2.5 equivalents of PAS-4200 gave the best product mixtures under these experimental conditions. (f) PAS derivatives do not affect the P50 values of DCLHb: the P50 values of polymerized product are in the range of 29 to 36 mm 15 Hg. (g) RP-HPLC analyses (Figure 13) indicate that both $- and o~a-chains are modified by PAS, but oca--ch~; n.s to a lesser extent than $-chains.
DCLHb polymerization by PAM derivatives may also be summarized. (a) As was true of the PAS
20 derivatives, the yield o~ oligomer increased with the number of molar equivalents of PAM used. (b) Elution times of the monomer decreased with the number of molar equivalents of PAM used; thus, decoration of DCLHb by PAM is likely. (c) Two equivalents of PAM
25 give the best product mixtures. (d) RP-HPLC profiles (Figure 15) suggest that reagent reacted specifically.
A specific $'-peak, which could be a modified $-peak, was detected at all ratios of PAM tested. Specific reaction with the subunits was also supported by the 30 decrease in titrable thiol residues. Reagent PAM is expected to bind specifically to cysteine-$93 residues, and about 65% and 90% of thiol groups are modified when 1 and 2 ec[uivalents of PAM are used, respectively. (e) The binding of PAM to the cysteine 35 residue results in a decrease in Pso values of the polymerized products to 18 to 20 mm Hg. (f) ococ-WO 95/17886 2 ~ 5 ~ ~ 2 ~ PCT/US94/14821 1~

~h~;ns are also modified, but much less extensively than the ~-~h~, n.~ .

BIQLOGICAL TESTING
In examples 8 through 12 we quenched the polyamide PAM-4200 by reaction with N-acetyl-L-cysteine and tested a sterile, non-pyrogenic solution of the polyamide (PAM-4080) in Ringer's lactate solution. The polyamide concentration was 5 g/dL of solution. The pH of the polyamide solution was adjusted to physiologic values. The osmolality of the solution was within the physiologic range. The concentration of the polyamide was selected to exceed projected use levels by at least an order of magnitude.

Exam~le 8 In vitro exposure of isolated mammalian cells.
CCL 1 NCTC 929 (clone of strain L cells, mouse connective tissue) were cultured aseptically in sterile media until confluency. The L-929 cell concentration was adjusted to about 1. 3 x 105 cells/mL, and aliquots were transferred to wells of a tissue culture plate. The plates were covered and incubated for approximately twenty four hours. Then the culture medium was aspirated from each well and aliquots of the test article solution and dilutions having PAM-4080 concentrations of 2.5 and 1 g/dL, respectively, were added to duplicate wells of the prepared plates. After incubation of the plates for approximately forty eight hours, the wells were stained with 2% crystal violet stain. The toxicity was rated on a scale from 0 to 4+, where a rating of 0 corresponded to the presence of discrete intracytoplasmic granules and the absence of cell lysis and a rating of 4+ corresponded to nearly 2 ~ 2 4 WO9S/17886 - 31 - PCT~S94/14821 complete destruction of the cell layers. At the highest concentration, a moderate toxicity rating of 2+ applied. At the two lower concentrations, a toxicity rating of 0 applied, i.e., the polyamide caused no adverse biological response.
No toxicity was observed at the lower doses and moderate toxicity was observed at the highest dose.
Accordingly, the polyamides of the present invention are expected to be nontoxic when ~mini stered as conjugates of therapeutically useful substrates.

.~xam~le 9 Acute toxicitv testin~ in rodents. Doses of 500 or 1500 mg of quenched PAM-4080/kg body weight were infused at a rate of 1 mL/kg/min. into the tail vein of male, Sprague-Dawley rats. Each test group consisted of six ~nim~l s; six undosed animals served as controls. All ~nim~ls were monitored for seventy two hours for signs of overt toxicity; none were observed. The ~nim~l s were sacrificed. No evidence of toxicity was seen at the time of necropsy. Tissues from the liver, kidney, lung were subjected to histopathological analysis. No adverse histopathology findings were noted.

F.xample 10 Com~atibilitY with human ervthrocytes. To determine the biocompatibility of PAM-4080 with human erythrocytes, the stock polyamide solution was diluted five-fold with lactated Ringer's solution. A volume of this preparation was mixed with an equal volume of heparinized human blood, vortexed gently, and placed in an incubator (37C) overnight. After an incubation period of 16 hours, a 100-~L ali~uot of the supernatant was removed from the top of the test sample; care was taken not to disturb the sedimented WO95/17886 ~b~2~:-` PCT~S94/14821 -red cells below. The aliquot was mixed with 5000 ~L
of SEC mobile phase, filtered through a 0.2 ~m pore-size filter and injected on a SuperoseTM 12 column for SEC analysis for native hemoglobin. The experimental data indicated that less than 0.1% hemolysis had occurred. This amount of hemolysis was considered negligible.

Ex~mnle ll Com~atibilitv with human ~eri~heral blood mononuclear cells (monocvtes). The potential of PAM-4080 for causing white blood cell activation was evaluated. The stock polyamide solution was diluted five-fold with lactated Ringer's solution. A volume of this preparation was mixed with an equal volume of peripheral blood mononuclear cell preparation and vortexed gently. An aliquot of this test preparation was removed and diluted with trypan blue. Toxicity was determined by microscopic detection of cells that could no longer exclude the dye. Percent viability was measured by a ratio of live/dead cells. PAM-4080 caused no decrease in cell viability. The remaining test preparation was placed in an incubator (37C) overnight. After an incubation period of 16 hours, cytokines were analyzed by pipetting an aliquot of the sample into microtiter wells and quantitation by ELISA. The concentrations of Tumor Necrosis Factor (TNF), Interleukin-l~ and Interleukin-6 determined were no different from those found by exposure of human monocytes to lactated Ringer's solution. Thus, PAM-4080 is compatible with human monocytes.

WO95/17886 21~ 6 9~24 PCT~S94114821 Exam~le 12 Com~atibilitv of PA-DCLHb with human ~eri~heral blood mononuclear cells (monocYtes). The potential of polyamide decorated and polymerized DCLHb (PA-DCLHb) to induce cytokine production by human monocytes was evaluated. Lactated Ringer's solution was used as the control article. The test articles were seven different preparations of PA-DCLHb in lactated Ringer's solution. Test and control solutions were made by mixing a volume of each test and control article with an equal volume of peripheral blood mononuclear cell preparation. After incubation of each resulting test and control solution at 37C for about 16 hours, an aliquot of each sample was transferred into separate wells of microtiter plates and the concentrations of Tumor Necrosis Factor (TNF), Interleukin-l~ and Interleukin-6 were quantitated by ELISA. The concentrations of each cytokine determined are shown in the Table below. The experimental data indicate that induction of TNF, IL-l, and IL-6 are low and in some cases comparable to Ringers. In summary, PA-DCLHb appears to be very compatible with human monocytes.

WO95/17886 2 ~ ~ ~ 9 ~ i PCT~S94/14821 -CYTOKINE CONCENTRATION, ng~mL
TEST ARTICLE
TNF IL-1~ IL-6 Lactated Ringer's 0.044 i 0.006 i c Solution (Control) 0.023 0.005 Detection Limit (DL) PA-DCLHb 0.154 i 0.080 i < DL
(Preparation 1) 0.027 0.040 PA-DCLHb 0.249 i 0.073 i < DL
(Preparation 2) 0.081 0.028 PA-DCLHb 0.161 i 0.054 i < DL
(Preparation 3) 0.055 0.011 PA-DCLHb 0.173 i 0.058 i < DL
(Preparation 4) 0.043 0.012 PA-DCLHb 0.139 i 0.049 + < DL
(Preparation 5) 0.027 0.009 PA-DCLHb 0.159 + 0.042 + < DL
(Preparation 6) 0.012 0.026 PA-DCLHb 0.144 i 0.048 i < DL
(Preparation 7) 0.050 0.028 Fxample 13 Cvtokine Induction bY PAS-DCLHb.
Samples of six PAS-DCLHb product mixtures were submitted for cytokine testing. The products selected were prepared by polymerization of 3 g/dL DCLHb in 0.lM HEPES buffer at pH 7Ø Each sample was diluted to a DCLHb concentration of about 1 g/dL and passed through an END-XTM endotoxin-removing filter. The filtrate was tested for cytokine induction using the method described in Example 12.

TEST SAMPLE TNF- , IL-1~, IL-6, ng/mL nq/mL ng/mL
Lactated Ringer's 0.044 0.006 0.044 Solution PAS-DCLHb (:::) 0.1,4 0.080 0.008 PAS-DCLH~ (~ ) o.^~c 0.07 0 PAS-DCLH~ ( ::) 0.:~: 0.0 L_ O . 001 PAS-DCLH~ (~::) 0. 'l- 0.0 0.0:7 PAS-DCLH~ (7::) O. 3r~ O.OL r` O.O 6 PAS-DCLH~ (~::) 0. 5~ 0.0~2 0.0_~
PAS-DCLH~ ( 0:1) 0. 4~ 0.0~8 0.O

WO95/17886 2 1 5 6 9 2 4 PCT~S94/14821 PAS-DCLHb (3:l) is the least decorated and polymerized product mixture, whereas PAS-DCLHb (lO:l) is the most ~ extensively decorated and polymerized product mixture.
The extent of decoration and polymerization increases with the molar ratio of PAS employed. However, the PAS-Hb products, irrespective of the extent of decoration or polymerization, all yield low TNF- and IL-l responses. None of the samples show an IL-6 response.
Exam~le 14 Svnthesis of Thio-containinq ~olvamide As a part of this work, five experimental parameters were studied: (l) the molar ratio of monomers (diester and diamine); the solvent; the reaction temperature; the order of mixing; and the method of product isolation. The objective of these studies was the identification of reaction conditions that would reproducibly maximize the yield of polymers having specific molecular weights. The molar ratios of diester to diamine were varied from l:l to l:l.4.
The solvents studied included chloroform and DMF. The basic catalyst was varied from 2,6-lutidine (a mild base) to triethylamine (a strong base) to no added catalyst. The temperature ranged from -50 C to room temperature (approximately 23 C). The diester was added to the diamine or vice versa. The rate of mixing was controlled by varying the rate of stirring of the solution, by varying the rate of addition, or by controlling the solubility of one of the components (the diester). It was found that product isolation was facilitated and polymer yield was improved by conversion of a polyamide bis(diamine) to a polyamide bis(succinate).
As a result of this study, it was found that water-soluble polyamides having molecular weights of ~ ` ~
WO95/17886 " ~ " PCT~S94/14821 -approximately 2800 and 5700 could be prepared selectively by polycondensation of TBB (3,3_-thiodipropionate active ester) with DGBE [diethylene glycol bis(3-aminopropyl ether); the diamine] under the conditions described in the Table. In both cases, the polycondensation reaction re~uired 4-24 hours, depending on scale, and the yield of polyamide approximated or exceeded 50%.
Table. Optimum conditions for the polycondensation of TBB and DGBE to yield water-soluble polyamides having specific molecular weights 2~ 692~
WO95/17886 ; PCT~S94/14821 Svnthesis of DiPhenvl (2,3-dihvdro-2-thioxo-3-benzoxazoYl)~hos~honate (DDTBP). To a solution of 2-mercaptobenzoxazole (251.6 g, 1.66 mole) and triethylamine (191.4 g, 1.89 mol) in 1 liter of toluene was added dropwise at room temperature with stirring a solution of diphenyl chlorophosphate (505.1 g, 1.88 mole) in 400 mL toluene. After the addition was completed, the solution was stirred for an additional 1.5 hours, during which time a precipitate formed. Thin-layer chromatographic analysis (TLC;
silica gel; eluent: ethyl ether/hexane, 1:1, v/v) of the reaction mixture indicated complete reaction. The solid was removed by filtration and washed with toluene (3 x 100 mL). The combined filtrates were evaporated to a residual oil. The oil was taken up in 500 mL of chloroform and the resulting solution was heated at reflux for about an hour. The solution was passed through a pad of silica gel. The pad was washed with chloroform until TLC analysis of the ~iltrate indicated that the product was completely eluted from the silica gel. The chloroform solution was evaporated, leaving as a solid the desired product. Hexane (1.5 L) was added, and the solid was collected by filtration and dried under vacuum. The product, 582.0 g of a white solid identified by the acronym DDTBP, was characterized by a melting point of 80-83 C (uncorrected) and the following NMR
resonances.
1H-NMR (CDCl3): 7.21 (m, 4), 7.35 (m, 9) and 7.91 (m, 1) ppm.
13C-NMR (CDC13): 109.9 (s, C9), 114.8 (s, C8), 120.1-120.3 (overlapping singlets, C2), 125.5 (s, C7), 126.3 (s, C10), 129.9-130.0, overlapping singlets, C3), 147.5 (s, C5), 149.5 (s, C1), and 180.2 (s, C11) ppm.

~ .

WO95/17886 6 9 2 1 PCT~S94/14821 31P-NMR (CDCl3): -16.17 ppm (with a minor impurity at -8.9 ppm) SYnthesis of N,N~-(3 3~-thiodi~ro~ionvl)bis(benzoxazoline-2-thione) (TBB). To a stirred solution of 3,3'-thiodipropionic acid (891 - mg, 5 mmol) and triethylamine (1.5 mL) in chloroform (20 mL) was added DDTBP (4.22 g, 11 mmol). The solution was stirred at room temperature and monitored by TLC (silica gel; eluent: ethyl ether/hexane, 1:1, v/v). With time, the product began to precipitate from solution. Methanol (100 mL) was added to facilitate complete precipitation of the product, which was isolated by filtration and air-dried. About 1.7 g (76%
of theoretical) of the product, N,N'-(3,3'-thiodipropionyl)bis(benzoxazoline-2-thione) or TBB, was obtained as a white solid having a melting point (uncorrected) of 147-149-C.
1H-NMR (CDCl3): 3.07 (t, H1), 3.89 (t, H2), 7.27, 7.32, 7.37 (H4, Hs, H6) and 8.08 (t, H3) ppm.
13C-NMR (CDCl3): 22.65 (C2), 39.91 (C1), 109.58, 116.4 (C4, Cs), 125.5, 126.17 (C3, C6), 129.6 (Cg), 146.41 (C7), 172.22 (C1o), and 178.46 (Cg) ppm.
Svnthesis of PATS-2800, a water-soluble ~olYamide havina a number averaae molecular weiaht of about 2800 Daltons. A slurry of TBB (5.34 g, 12 mmol) in 60 mL
chloroform was stirred at a moderate rate while being cooled to 0 in an external ice-bath as a solution of DGBE (3.17 g, 1.4 mmol, a 1.2:1 molar ratio relative to TBB) in 12 mL chloroform was added. The resulting mixture was stirred for 15 minutes at 0-5 C and then the ice-bath was removed. Stirring continued at ambient temperatures overnight. Thin-layer chromatographic analysis indicated that a polyamide bis(amine) had formed.

215~924 WO95/17886 PCT~S94114821 A solution of succinic anhydride (850 mg) in 3 mL
DMF was added gradually to the polymer solution until thin-layer chromatographic analysis indicated all the polyamide bis(amine) had been converted to the corresponding polyamide bis(carboxylic acid).
Volatile materials were removed from the reaction mixture by evaporation to dryness under vacuum, and the residue was taken up in 20 mL DMF. Then volatile materials were removed by evaporation under vacuum.
The residue was dissolved in a second, 20-mL portion of DMF. Ethyl acetate was added slowly to the resulting solution; precipitation of the product appeared to be complete after the addition of about 300 mL of ethyl acetate. The product was collected by filtration, washed with ethyl acetate and dried under high vacuum. About 2.27 g (47% of theoretical) of water-soluble polyamide (identified by the acronym PATS) having a number average molecular weight (based on NMR analysis) of 2800 Daltons and a size exclusion chromatographic (SEC) retention time of 38.8 minutes was obtained.
SYnthesis of PATSS-2800, an activated, water-soluble ~olvamide havina a number avera~e molecular wei~ht of about 2800 Daltons. N,N'-Disuccinimidyl carbonate (1.18 g, 6.42 mmol~ was added to a stirred solution of PATS-2800 (1.96 g, 0.7 mmol) in a mixture of 10 mL DMF and 30 mL chloroform. The mixture was stirred at room temperature and the reaction was followed by TLC (silica gel; eluent:
CHCl3/MeOH/NH4OH/H2O, 10:3:0.2:0.2, by volume). After 3,5 hours, the reaction mixture was filtered to remove insoluble materials. The filtrate was concentrated under vacuum to dryness. The residue was dissolved in 15 mL DMF and the solution was diluted slowly with ethyl acetate (300 mL) to precipitate the product, a bis(N-oxysuccinimidyl) polyamidedicarboxylate which is WO95/17886 ~ l 56~ PCT~S94/14821 identified by the acronym PATSS-2800. The product (1.52 g, 77% yield) was isolated by filtration and dried under high vacuum.
1H-NMR (CDCl3): 1.71 (m, Hb); 2.39 (m, Hg); 2.52 (t, Hs or Ht); 2.76 (m); 2.78 (Hf, Hh); 2.90 (t, Hs or Ht); 3.27 (m, Ha); 3.47-3.57 (m, Hc, Hd); 6.78 (CONH) ppm.
13C-NMR (CDCl3): 25.5 (Cr); 26.7; 30.3 (Cs, Ct);
27.7 (Cg); 28.9 (Cb); 36.4 (Cf); 37.5 (Ca); 69.5;
69.9; 70.3 (Cc, Cd); 168.1, 169.0; 169.8; and 171.2 (C=O) ppm. (NOTE: Not all resonances have been correlated with specific structural sites.) Absorbance ratioing indicated the number average molecular weight of the polymer was about 2800 Daltons.
Svnthesis of PATS-5700, a watex-soluble olYamide havina a number averaae molecular weiaht of about S700 Daltons. To a slurry of TBB (5.34 g, 12 mmol) in 60 mL DMF that was being stirred at a moderately slow rate was added a solution of DGBE (3.44 g, 1.68 mmol, a 1.3:1 molar ratio relative to TBB) in 6 mL DMF. The solid gradually dissolved and the mixture became warm.
The resulting solution was stirred at room temperature overnight. A precipitate gradually separated from the solution. The precipitate (2.44 g; about 47% of theoretical) was isolated by filtration and was found to have a SEC retention time of about 35.8 minutes and was characterized by TLC as a polyamide monoamine monocarboxylate having an average molecular weight of about 5700 Daltons. The filtrate was found to contain a polymer (1.14 g; 22% of theoretical) having a SEC
retention time of about 38.6 minutes (i.e., the polyamide bis(amine) had a number average molecular weight of about 2800 Daltons).

WO95/17886 ~ ~ ~ 6 ~ ~ 4 PCT~S94/14821 SYnthesis of PATSS-5700, an activated water-soluble ~olvamide havina a number averaae molecular weiaht of about 2800 Daltons. The above precipitate (2.44 g) was dissolved in 60 mL chloroform and about 3 mL methanol was added to ensure complete dissolution.
Then volatile materials were removed under vacuum to ensure complete removal of residual DMF. The solid was dissolved in a second, 60-mL portion of chloroform. To the resulting solution was added succinic anhydride (108 mg) in 1 mL DMF. Reaction was monitored by TLC. Stirring was continued until all polyamide amine had been converted to polyamide bis(carboxylic acid). To this solution was added successively triethylamine (about 400 ~L), 10 mL DMF
and 730 mg N,N'-disuccinimidyl carbonate. The mixture was stirred at room temperature and the reaction was followed by TLC. After 2.5 hours, volatile materials were removed under vacuum and the residual solid was dissolved in 10 mL DMF. The solution was slowly diluted with ethyl acetate (100 mL) to precipitate the product, bis(N-oxysuccinimidyl) polyamidedicarboxylate, identified by the acronym PATSS-5700. About 2.36 g of product was isolated by filtration and dried under vacuum.
13C-NMR (CDC13): 25.5 (Cr); 26.8; 30.4 (Cs, Ct);
27.7 (Cg); 29.0 (Cb); 36.5 (Cf); 37.6 (Ca); 69.6;
70.0; 70.4 (Cc, Cd); 168.2, 169.1; 169.9; and 171.3 (C=O) ppm. (NOTE: Not all resonances have been correlated with specific structural sites.) Absorbance ratioing indicated the number average molecular weight of the polymer was about 5700 Daltons.
As will be readily appreciated, numerous variations and combinations of the features set forth above can be utilized without departing from the present invention as set forth in the claims. All ~ 4' PCT~S94/14821 -Wo95/17886 such variations are intended to be included in the scope of the following claims.

Claims (42)

CLAIMS:
1. A water-soluble, substantially nonimmunogenic polyamide selected from the group consisting of:
I Y-A-X-Y
II Z-B-X-Z
III Y-X-Z
(a) where terminus Y is OH or a carboxyl coupling group;
(b) where terminus Z is H or a coupling group attached to an amine group; and (c) where X is a polyamide selected from:
(B-A)n, (A-B)n, and branched polyamides formed by linking (B-A)n or (A-B)n to a central polyacid, polyamine or polyamino acid; and (d) where A is a .alpha.,.omega.-di-acid; B is a .alpha.,.omega.-diamine; n is the number of amide repeat units in the polyamide; and (e) where the acid subunits of the amide repeat units are two or more organic acids each of said organic acids having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N present as substituents on or atoms in the chain bridged by a water-soluble diamine having the formula -NH-R1-NH- where R1 is a substituted or unsubstituted aliphatic chain having from about 4 to about 5 carbon atoms; and (f) where the amine subunits of the amide repeat units are organic, water-soluble amines having at least one primary amine group and having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O
other than carboxyl or carbonyl O, S, P or N present as substituents on or atoms in the chain; and (g) where n is from 2 to about 100.
2. A polyamide of Claim 1 wherein the water-soluble diamine having the formula -NH-R1-NH- is 1,4 diaminobutane.
3. Two or more polyamides of Claims 1 or 2 linked by a central polyacid, polyamine or polyamino acid to form branched, water-soluble polyamides.
4. A polyamide of Claims 1 or 2 reacted with a substrate having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides; steroids;
and carbohydrates; wherein the product of said reaction is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
5. A polyamide of Claims 1 or 2 decorating a substrate having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said decorating is water-soluble, substantially nonimmunogenic, and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
6. A polyamide of Claims 1 or 2 cross-linking two or more substrates having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said cross-linking is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
7. A polyamide of Claims 1 or 2 polymerizing three or more substrates having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said polymerizing is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
8. A polyamide of Claims 1 or 2 decorating a product of Claim 7.
9. A polyamide of Claims 1 or 2 decorating a product of Claim 6.
10. A product of Claim 7 wherein said substrates are hemoglobin molecules and wherein said polyamide is bis(maleimidoacyl) polyamide.
11. A product of Claim 7 wherein said substrates are hemoglobin molecules and wherein said polyamide is bis(N-oxa-succinimidyl) polyamide.
12. Water-soluble, substantially nonimmunogenic branched or straight chain polyamides having number average molecular weights of about 300 to about 20,000 grams per mole; comprising from 1 to about 100 amide repeat units where each repeat unit comprises:
(a) a water-soluble organic acid having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N present as substituents on or atoms in the chain bridged by a water-soluble diamine having the formula -NH-R1-NH- where R1 is a substituted or unsubstituted aliphatic chain having from about 4 to about 5 carbon atoms; and (b) covalently linked as an amide to;

(c) a water-soluble organic amine subunit having at least one primary amino group and fifteen or fewer atoms separating the amide functionalities in the polyamide.
13. A polyamide of Claim 1 where terminus Y and terminus Z are independently activated by reacting said polyamide with bi- or polyfunctional protein reagents selected from the group consisting of dialdehydes, N-hydroxysuccinimide esters, activated esters, functionalized acetals, bis-maleimides, bifunctional imino esters, diepoxides, and dicarboxylic acid chlorides.
14. A water-soluble, substantially nonimmunogenic polyamide selected from the group consisting of:
I Y-A-X-Y
II Z-B-X-Z
III Y-X-Z
(a) where terminus Y is OH or a carboxyl coupling group;
(b) where terminus Z is H or a coupling group attached to an amine group; and (c) where X is a polyamide selected from:
(B-A)n, (A-B)n, and branched polyamides formed by linking (B-A)n or (A-B)n to a central polyacid, polyamine or polyamino acid; and (d) where A is a .alpha.,.omega.-di-acid; B is a .alpha.,.omega.-diamine; n is the number of amide repeat units in the polyamide; and (e) where the acid subunits of the amide repeat units are organic acids having the formula where m is from about 2 to about 4, X1 and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or N, and R2 is H or acetamide;
(f) where the amine subunits of the amide repeat units are organic, water-soluble amines having at least one primary amine group and having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of carboxyl or carbonyl O, S, P or N present as substituents on or atoms in the chain; and (g) where n is from 2 to about 100.
15. A polyamide of Claim 14 wherein X1 and X2 are both S.
16. A polyamide of Claim 14 wherein X1 and X2 are both O.
17. A polyamide of Claim 14 wherein m is 2, and X1 and X2 are both O.
18. Two or more polyamides of Claim 14 or 17 linked by a central polyacid, polyamine or polyamino acid to form branched, water-soluble polyamides.
19. A polyamide of Claims 14 or 17 reacted with a substrate having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides; steroids;
and carbohydrates; wherein the product of said reaction is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
20. A polyamide of Claims 14 or 17 decorating a substrate having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said decorating is water-soluble, substantially nonimmunogenic, and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
21. A polyamide of Claims 14 or 17 cross-linking two or more substrates having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said cross-linking is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
22. A polyamide of Claims 14 or 17 polymerizing three or more substrates having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said polymerizing is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
23. A polyamide of Claims 14 or 17 decorating a product of Claim 22.
24. A polyamide of Claims 14 or 17 decorating a product of Claim 21.
25. A product of Claim 23 wherein said substrates are hemoglobin molecules and wherein said polyamide is bis(maleimidoacyl) polyamide.
26. A product of Claim 23 wherein said substrates are hemoglobin molecules and wherein said polyamide is bis(N-oxa-succinimidyl) polyamide.
27. Water-soluble, substantially nonimmunogenic branched or straight chain polyamides having number average molecular weights of about 300 to about 20,000 grams per mole; comprising from 1 to about 100 amide repeat units where each repeat unit comprises:
(a) organic acids having the formula where m is from about 2 to about 4, X1 and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N, and R2 is H or acetamide;
(b) covalently linked as an amide to;
(c) a water-soluble organic amine subunit having at least one primary amino group and fifteen or fewer atoms separating the amide functionalities in the polyamide.
28. A polyamide of Claim 14 or 17 where terminus Y and terminus Z are independently activated by reacting said polyamide with bi- or polyfunctional protein reagents selected from the group consisting of dialdehydes, N-hydroxysuccinimide esters, activated esters, functionalized acetals, bis-maleimides, bifunctional imino esters, diepoxides, and dicarboxylic acid chlorides.
29. A water-soluble, substantially nonimmunogenic polyamide selected from the group consisting of:
I Y-A-X-Y
II Z-B-X-Z
III Y-X-Z
(a) where terminus Y is OH or a carboxyl coupling group;
(b) where terminus Z is H or a coupling group attached to an amine group; and (c) where X is a polyamide is selected from the group consisting of: (B-A')n or (A'-B)n and branched polyamides formed by linking (B-A')n or (A'-B)n to a central polyacid, polyamine or polyamino acid; and (d) where B is a .alpha.,.omega.-diamine; n is the number of amide repeat units in the polyamide; and A' is a .alpha.,.omega.-di-acid having the formula where Y1 has the formula -OC-(CH2)p-NH-where p is from 1 to about 4, m is from about 2 to about 4, X1 and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N, and R3 is a lower alkyl having from about 1 to about 2 carbon atoms;
(e) where the amine subunits of the amide repeat units are organic, water-soluble amines having at least one primary amine group and having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O
other than carboxyl or carbonyl O, S, P or N present as substituents on or atoms in the chain; and (f) where n is from 2 to about 100.
30. A polyamide of claim 29 wherein X1 and X2 are both O, m is 2, and R3 is methyl.
31. Two or more polyamides of Claims 29 or 30 linked by a central polyacid, polyamine or polyamino acid to form branched, water-soluble polyamides.
32. A polyamide of Claims 29 or 30 reacted with a substrate having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides; steroids;
and carbohydrates; wherein the product of said reaction is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
33. A polyamide of Claims 29 or 30 decorating a substrate having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said decorating is water-soluble, substantially nonimmunogenic, and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
34. A polyamide of Claims 29 or 30 cross-linking two or more substrates having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said cross-linking is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
35. A polyamide of Claims 29 or 30 polymerizing three or more substrates having a diagnostic or therapeutic biological activity selected from the group consisting of proteins including enzymes, haptens, and antibodies; polypeptides; polynucleotides including probes; and carbohydrates; wherein the product of said polymerizing is water-soluble, substantially nonimmunogenic and retains a diagnostically or therapeutically useful amount of the substrate's biological activity.
36. A polyamide of Claims 29 or 30 decorating a product of Claim 35.
37. A polyamide of Claims 29 or 30 decorating a product of Claim 34.
38. A product of Claim 35 wherein said substrates are hemoglobin molecules and wherein said polyamide is bis(maleimidoacyl) polyamide.
39. A product of Claim 35 wherein said substrates are hemoglobin molecules and wherein said polyamide is bis(N-oxa-succinimidyl) polyamide.
40. Water-soluble, substantially nonimmunogenic branched or straight chain polyamides having number average molecular weights of about 300 to about 20,000 grams per mole; comprising from 1 to about 100 amide repeat units where each repeat unit comprises:
(a) a water-soluble organic acid having the formula where Y1 has the formula -OC-(CH2)p-NH-where p is from 1 to about 4, m is from about 2 to about 4, X1 and X2 are independently a heteroatom selected from the group consisting of O other than carboxyl or carbonyl O, S, P or tertiary N, and R3 is a lower alkyl having from about 1 to about 2 carbon atoms;
(b) covalently linked as an amide to;
(c) a water-soluble organic amine subunit having at least one primary amino group and fifteen or fewer atoms separating the amide functionalities in the polyamide.
41. A polyamide of Claim 29 or 30 where terminus Y and terminus Z are independently activated by reacting said polyamide with bi- or polyfunctional protein reagents selected from the group consisting of dialdehydes, N-hydroxysuccinimide esters, activated esters, functionalized acetals, bis-maleimides, bifunctional imino esters, diepoxides, and dicarboxylic acid chlorides.
42. A water-soluble, substantially nonimmunogenic polyamide selected from the group consisting of:
I Y-A-X-Y
II Z-B-X-Z
III Y-X-Z
(a) where terminus Y is OH or a carboxyl coupling group;
(b) where terminus Z is H or a coupling group attached to an amine group; and (c) where X is a polyamide is selected from the group consisting of: (B-A')n or (A'-B)n and branched polyamides formed by linking (B-A')n or (A'-B)n to a central polyacid, polyamine or polyamino acid; and (d) where B is a .alpha.,.omega.-diamine; n is the number of amide repeat units in the polyamide; and A' is a .alpha.,.omega.-di-acid having the formula where Y1 has the formula - OC-(CH2)p-NH- ,where p is from 1 to about 4; and where A is an acid subunit of the amide repeat units having two or more organic acids each of said organic acids having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O
other than carboxyl or carbonyl O, S, P or tertiary N
present as substituents on or atoms in the chain bridged by a water-soluble diamine having the formula -NH-R1-NH- where R1 is a substituted or unsubstituted aliphatic chain having from about 4 to about 5 carbon atoms;
(e) where the amine subunits of the amide repeat units are organic, water-soluble amines having at least one primary amine group and having fifteen or fewer atoms in the chain and having one or more heteroatoms selected from the group consisting of O
other than carboxyl or carbonyl O, S, P or N present as substituents on or atoms in the chain; and (f) where n is from 2 to about 100.
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