A rapid method for determination of endoproteinase substrate specificity: specificity of the 3C proteinase from hepatitis A virus.

Petithory, Joanne R.; Masiarz, Frank R.; Kirsch, Jack F.; Santi, Daniel V.; Malcolm, Bruce A.

doi:10.1073/pnas.88.24.11510

Cited by 49 publications

(26 citation statements)

References 26 publications

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“…Ac-WRY-OMe, a fragment of the proteinaceous inhibitor tendamistat, binds with a K, value of 100 ,uM (T. Guo and P.A.B., unpublished data); the corresponding peptoids show similar affinity, with the retro sequence 9 (K, 200 AuM) preferred slightly over the direct-translation peptoid 8 (K, 350 AM). In another example, both forward, 6, and retro, 5, peptoid analogs ofthe consensus substrate (Ac-ELATQSFS-NH2) of the hepatitis A virus 3C protease (23,38) were prepared, with the "conservative" substitution of Nhser for threonine. While the retro peptoid, 5 (K, 2 mM), competed with affinity comparable to that of the peptide substrate (Km 2.1 mM), the forward peptoid, 6, showed no inhibition at 10 mM concentration.…”

Section: Methodsmentioning

confidence: 99%

Peptoids: a modular approach to drug discovery.

Simon¹,

Kania²,

Zuckermann³

et al. 1992

Proc. Natl. Acad. Sci. U.S.A.

914

636

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Peptoids, oligomers ofN-substituted glycines, are described as a motif for the generation ofchemically diverse libraries of novel molecules. Ramachandran-type plots were calculated and indicate a greater diversity of conformational states available for peptoids than for peptides. The monomers incorporate t-butyl-based side-chain and 9-fluorenylmethoxycarbonyl a-amine protection. The controlled oligomerization of the peptoid monomers was performed manually and robotically with in situ activation by either benzotriazol-lyloxytris(pyrrolidino)phosphonium hexafluorophosphate or bromotris(pyrrolidino)phosphonium hexafluorophosphate. Other steps were identical to peptide synthesis using a-(9-fluorenylmethoxycarbonyl)amino acids. A total of 15 monomers and 10 oligomers (peptoids) are described. Preliminary data are presented on the stability of a representative oligopeptoid to enzymatic hydrolysis. Peptoid versions of peptide ligands of three biological systems (bovine pancreatic a-amylase, hepatitis A virus 3C proteinase, and human immunodeficiency virus transactivator-responsive element RNA) were found with affinities comparable to those of the corresponding peptides. The potential use of libraries of these compounds in receptor-or enzyme-based assays is discussed.Broad screening of compound libraries, of broths grown from soil samples, and of synthetic intermediates has been a fruitful method for discovery of lead compounds in pharmaceutical and agrochemical research (e.g., ref. 1). With the advent of automated chemical methods for solid-phase peptide and nucleotide synthesis, and of molecular biological methods for protein and nucleic acid synthesis, the stage has been set for the generation of new kinds of compound libraries, namely, collections of oligomeric biomolecules (2-14). Such libraries have been used to map epitopes for antibody binding, to discern ribonucleotide sequences with specific binding or catalytic activity, and to provide initial leads in receptor-based assays. Advantages of these oligomeric molecules are an almost limitless diversity as a result of their modular structure, the ease with which they can be synthesized and sequenced, and their inherent biological relevance. On the other hand, the metabolic instability of peptides and nucleotides and their poor absorption characteristics mean that any lead sequence will require extensive modification before in vivo activity can be expected.Many of these problems could be avoided if an alternative, modular system was devised, with a basis set of "unnatural" monomers and a method for their controlled oligomerization. A host of chemically and pharmaceutically interesting subunits or modules would generate a diverse and novel set of heteropolymers. Once an interesting compound has been identified from a library of such nonpeptide polymers, it can serve as a lead for drug discovery, further along the road to a metabolically stable drug. Optimized analogs of a lead compound could then be developed rapidly due to the modular synthetic nature of th...

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Section: Methodsmentioning

confidence: 99%

Peptoids: a modular approach to drug discovery.

Simon¹,

Kania²,

Zuckermann³

et al. 1992

Proc. Natl. Acad. Sci. U.S.A.

914

636

View full text Add to dashboard Cite

show abstract

“…The biological method involves the display of the peptide libraries on filamentous phage, the identification of the best substrates by molecular biology tools, and the cleavage site determination in each substrate [1][2][3][4]. Synthetic peptide libraries can contain millions of compounds, but the identification of the substrates and the cleavage site require robust analytical assays such as Edman degradation [5][6][7], mass spectrometry [8,9], and chromatography [10]. Support-bound fluorescence resonance energy transfer (FRET) 1 peptide libraries have been prepared by the process of split synthesis, resulting in a single peptide sequence on each of the resin beads [11].…”

mentioning

confidence: 99%

Positional-scanning combinatorial libraries of fluorescence resonance energy transfer peptides to define substrate specificity of carboxydipeptidases: assays with human cathepsin B

Cotrin

Puzer

Júdice

et al. 2004

Analytical Biochemistry

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“…Determined by Peptide Libraries-Peptide libraries were used to identify preferred amino acids of substrates at or near the cleavage site and to map the primed subsite 2 binding region of meprins (25). A completely random dodecapeptide mixture acetylated at the amino terminus was partially digested with meprin A or B, and the digested peptides were subjected to amino-terminal peptide sequencing.…”

Section: Meprin a And B Have Distinct Specificities For Preferred Amimentioning

confidence: 99%

Marked Differences between Metalloproteases Meprin A and B in Substrate and Peptide Bond Specificity

Bertenshaw¹,

Turk²,

Hubbard³

et al. 2001

Journal of Biological Chemistry

105

112

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Meprin A and B are highly regulated, secreted, and cell-surface metalloendopeptidases that are abundantly expressed in the kidney and intestine. Meprin oligomers consist of evolutionarily related ␣ and/or ␤ subunits. The work herein was carried out to identify bioactive peptides and proteins that are susceptible to hydrolysis by mouse meprins and kinetically characterize the hydrolysis. Gastrin-releasing peptide fragment 14 -27 and gastrin 17, regulatory molecules of the gastrointestinal tract, were found to be the best peptide substrates for meprin A and B, respectively. Peptide libraries and a variety of naturally occurring peptides revealed that the meprin ␤ subunit has a clear preference for acidic amino acids in the P1 and P1 sites of substrates. The meprin ␣ subunit selected for small (e.g. serine, alanine) or hydrophobic (e.g. phenylalanine) residues in the P1 and P1 sites, and proline was the most preferred amino acid at the P2 position. Thus, although the meprin ␣ and ␤ subunits share 55% amino acid identity within the protease domain and are normally localized at the same tissue cell surfaces, they have very different substrate and peptide bond specificities indicating different functions. Homology models of the mouse meprin ␣ and ␤ protease domains, based on the astacin crystal structure, revealed active site differences that can account for the marked differences in substrate specificity of the two subunits.Meprin A and B are zinc metalloendopeptidases composed of evolutionarily related ␣ and/or ␤ subunits. They are members of the astacin family and are highly expressed in brush border membranes of the intestine and renal proximal tubules (1, 2). Meprins are particularly abundant in mouse juxtamedullary nephrons and constitute ϳ5% of total protein in renal brush border membranes (3). The meprin ␣ and ␤ subunits are expressed early in embryonic development of mouse kidney and intestine, by day 11, and have different patterns of expression in the suckling phase and after weaning (4). Homologous enzymes are found in rat and human kidney and intestine (1,5,6). Meprins are also expressed in leukocytes of intestinal lamina propria and in cancer cells and are consequently implicated in inflammation and cancer growth and metastasis (7,8).Mouse kidney meprin A (EC 3.4.24.18) is a homooligomer of ␣ subunits, or a heterooligomer of ␣ and ␤ subunits (2, 9). Mouse kidney meprin B (EC 3.4.24.63) is a homooligomer of ␤ subunits (10). The multidomain ␣ and ␤ meprin subunits are highly glycosylated and form disulfide-linked dimers and higher order oligomers by noncovalent interactions (11,12). Meprins containing at least one ␤ subunit remain membranebound by virtue of a transmembrane domain located near the carboxyl terminus of ␤ subunits (1). Mature meprin ␣ homooligomers contain no transmembrane domain and are found in mouse urine (13). The expression of the meprin ␣ subunits in mice is strain-dependent (1). Random-bred mice (such as ICR) and many inbred strains of mice (e.g. C57BL/6) express both meprin ␣ and ␤ in...

show abstract

A rapid method for determination of endoproteinase substrate specificity: specificity of the 3C proteinase from hepatitis A virus.

Cited by 49 publications

References 26 publications

Peptoids: a modular approach to drug discovery.

Peptoids: a modular approach to drug discovery.

Positional-scanning combinatorial libraries of fluorescence resonance energy transfer peptides to define substrate specificity of carboxydipeptidases: assays with human cathepsin B

Marked Differences between Metalloproteases Meprin A and B in Substrate and Peptide Bond Specificity

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