NMR solution structure of a novel hirudin variant HM2, N-terminal 1-47 and N64 → V + G mutant

Nicastro, Giuseppe; Baumer, Luca; Bolis, Giorgio; Tatò, Marco

doi:10.1002/(sici)1097-0282(199706)41:7<731::aid-bip3>3.0.co;2-q

Cited by 13 publications

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References 41 publications

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“…Due to its important pharmacological implications, the hirudin thrombin pair has been the object of thorough biochemical and structural studies. Indeed, the high‐resolution crystallographic structures of both free (Pineda et al 2004; Johnson et al 2005) and hirudin‐bound forms of thrombin are available (Rydel et al 1991), together with several NMR structures of full‐length and truncated hirudin forms (Haruyama and Wuthrich 1989; Szyperski et al 1992; Nicastro et al 1997). Hence, taking advantage of the synthetic procedure previously established (De Filippis et al 1995, 1998), we synthesized two NT‐containing analogs of hirudin fragment 1 47: the Y3NT analog, in which Tyr3 was replaced by NT, and the S2R/Y3NT analog, containing the double substitution Ser2 → Arg and Tyr3 → NT.…”

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confidence: 99%

3‐Nitrotyrosine as a spectroscopic probe for investigating protein–protein interactions

2006

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3-Nitrotyrosine (NT) is ;103 -fold more acidic than Tyr, and its absorption properties are strongly pH-dependent. NT absorbs radiation in the wavelength range where Tyr and Trp emit fluorescence (300-450 nm), and it is essentially nonfluorescent. Therefore, NT may function as an energy acceptor in resonance energy transfer (FRET) studies for investigating ligand-protein interactions. Here, the potentialities of NT were tested on the hirudin-thrombin system, a well-characterized protease-inhibitor pair of key pharmacological importance. We synthesized two analogs of the N-terminal domain (residues 1-47) of hirudin: Y3NT, in which Tyr3 was replaced by NT, and S2R/Y3NT, containing the substitutions Ser2 ! Arg and Tyr3 ! NT. The binding of these analogs to thrombin was investigated at pH 8 by FRET and UV/Vis-absorption spectroscopy. Upon hirudin binding, the fluorescence of thrombin was reduced by ;50%, due to the energy transfer occurring between the Trp residues of the enzyme (i.e., the donors) and the single NT of the inhibitor (i.e., the acceptor). The changes in the absorption spectra of the enzyme-inhibitor complex indicate that the phenate moiety of NT in the free state becomes protonated to phenol in the thrombin-bound form. Our results indicate that the incorporation of NT can be effectively used to detect protein-protein interactions with sensitivity in the low nanomolar range, to uncover subtle structural features at the ligand-protein interface, and to obtain reliable K d values for structure-activity relationship studies. Furthermore, advances in chemical and genetic methods, useful for incorporating noncoded amino acids into proteins, highlight the broad applicability of NT in biotechnology and pharmacological screening.

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confidence: 99%

3‐Nitrotyrosine as a spectroscopic probe for investigating protein–protein interactions

2006

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“…Hirudin is the most potent and specific inhibitor of αT (K d = 20‐200 fM) and is now used as an anticoagulant drug (Refludan). Hirudin HM2 variant from Hirudinaria manillensis , an hematophagous parasite of bovines, is formed by a compact N‐terminal region (amino acids 1‐47) and a flexible negatively charged C‐terminal tail (amino acids 48‐64) (4htc.pdb) . The N‐terminal domain is stabilized by three disulfide bonds and covers the protease active site by extensively penetrating into the enzyme specificity sites through its N‐terminal tripeptide (Figure C‐E).…”

Section: Incorporation Of Non‐coded Amino Acids For Sar Studies Of Himentioning

confidence: 99%

“…A, RP‐HPLC analysis of the time‐course kinetics of fully reduced HM2(1‐47) (R) to yield the folded species with the native disulfide bond topology (N). (Inset) Tube representation of the NMR solution structure of HM2(1‐47) . Disulfide bonds are indicated by yellow sticks.…”

Section: Incorporation Of Non‐coded Amino Acids For Sar Studies Of Himentioning

confidence: 99%

“…The inhibitory potency of the synthetic Hir(1‐47) analogs toward the procoagulant ( fast ) and anticoagulant ( slow ) form of αT was measured at 25°C by monitoring the release of p ‐nitroanilide ( p ‐NA) from the synthetic substrate (D)‐Phe‐Pro‐Arg‐ p ‐NA under salt conditions stabilizing the fast (0.2 M NaCl) or the slow (0.2 M ChCl) form of the protease (Figure ). The amino acid exchanges were designed starting from the NMR solution structure of HM2 and the crystallographic structure of hirudin‐αT complex …”

Section: Incorporation Of Non‐coded Amino Acids For Sar Studies Of Himentioning

confidence: 99%

“…Position 3 . Tyr‐3 in HM2(1‐47) has a well‐defined conformation both in the free and αT‐bound state . Tyr‐3 partially fills the apolar S3 site of the protease, which is shaped by Leu‐99, Ile‐174, and Trp‐215, and is highly conserved in the hirudin family .…”

Section: Incorporation Of Non‐coded Amino Acids For Sar Studies Of Himentioning

confidence: 99%

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Protein engineering by chemical methods: Incorporation of nonnatural amino acids as a tool for studying protein folding, stability, and function

et al. 2018

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Proteins are large complex biomolecules that act as the effectors of essentially all cell functions. Due to the intrinsic complexity of protein architecture at the microscopic level and the inadequacy of theoretical methods to predict protein reactivity (ie, folding, stability, and function), protein engineering has emerged as a valuable tool to investigate structure–stability–activity relationships in proteins and nowadays recombinant DNA technologies are the “gold standard” for site‐specifically manipulating a given protein chain. The usefulness of current mutagenesis techniques, however, is limited by the relatively poor chemical diversity of the 20 DNA‐coded amino acids, such that it is difficult to precisely assign the observed change of protein stability or function to the variation of a single physicochemical property at a protein site (ie, hydrophobicity, conformational propensity, polarizability, hydrogen bonding, etc). In this article, we report relevant examples from our laboratory showing that chemical methods, that is, enzyme‐catalyzed semisynthesis and stepwise solid‐phase synthesis, allow to conveniently incorporate non‐natural amino acids with “tailored” side chains into small proteins and thus effectively transfer the structure–activity relationship methodology, typical of the medicinal chemistry approach on small molecules, to the study of folding, stability, and molecular recognition in macromolecular protein systems.

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Protein Engineering with Noncoded Amino Acids: Applications to Hirudin

Filippis¹

2010

Pharmaceutical Sciences Encyclopedia

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The incorporation of noncoded amino acids into proteins has emerged as a novel and promising approach in protein science. Several different strategies are being pursued to incorporate noncoded amino acids, including peptide synthesis native chemical ligation, enzyme‐catalyzed semisynthesis, biosynthetic incorporation via auxotrophic bacterial strain expression, and nonsense suppression methodologies in cell‐free or whole‐cell expression systems. This article discusses the use of noncoded amino acids in structure‐activity relationship (SAR) studies of hirudin binding to thrombin, as well as the incorporation of noncoded analogs of tryptophan and tyrosine as spectroscopic probes for studying the hirudin‐thrombin interaction.

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NMR solution structure of a novel hirudin variant HM2, N-terminal 1-47 and N64 → V + G mutant

Cited by 13 publications

References 41 publications

3‐Nitrotyrosine as a spectroscopic probe for investigating protein–protein interactions

3‐Nitrotyrosine as a spectroscopic probe for investigating protein–protein interactions

Protein engineering by chemical methods: Incorporation of nonnatural amino acids as a tool for studying protein folding, stability, and function

Protein Engineering with Noncoded Amino Acids: Applications to Hirudin

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