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Crystal structure of fibrinogen-Aalpha peptide 1-23 (F8Y) bound to bovine thrombin explains why the mutation of Phe-8 to tyrosine strongly inhibits normal cleavage at Arg-16.与牛凝血酶结合的纤维蛋白原-Aα肽1-23(F8Y)的晶体结构解释了为什么苯丙氨酸8突变为酪氨酸会强烈抑制精氨酸16处的正常切割。
Biochem J. 1997 Sep 15;326 ( Pt 3)(Pt 3):815-22. doi: 10.1042/bj3260815.
2
Substitution of tyrosine for phenylalanine in fibrinopeptide A results in preferential thrombin cleavage of fibrinopeptide B from fibrinogen.在纤维蛋白肽A中用酪氨酸取代苯丙氨酸会导致凝血酶从纤维蛋白原中优先切割纤维蛋白肽B。
Biochemistry. 1998 Sep 29;37(39):13704-9. doi: 10.1021/bi981190h.
3
The structure of residues 7-16 of the A alpha-chain of human fibrinogen bound to bovine thrombin at 2.3-A resolution.
J Biol Chem. 1992 Apr 15;267(11):7911-20.
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Bovine thrombin complexed with an uncleavable analog of residues 7-19 of fibrinogen A alpha: geometry of the catalytic triad and interactions of the P1', P2', and P3' substrate residues.与纤维蛋白原Aα亚基7-19位残基不可裂解类似物复合的牛凝血酶:催化三联体的几何结构以及P1'、P2'和P3'底物残基的相互作用
Biochemistry. 1996 Oct 8;35(40):13030-9. doi: 10.1021/bi960656y.
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Thrombin-bound structures of designed analogs of human fibrinopeptide A determined by quantitative transferred NOE spectroscopy: a new structural basis for thrombin specificity.通过定量转移NOE光谱法测定的人纤维蛋白肽A设计类似物的凝血酶结合结构:凝血酶特异性的新结构基础
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High-resolution NMR studies of fibrinogen-like peptides in solution: interaction of thrombin with residues 1-23 of the A alpha chain of human fibrinogen.溶液中纤维蛋白原样肽的高分辨率核磁共振研究:凝血酶与人纤维蛋白原Aα链1-23位残基的相互作用。
Biochemistry. 1989 Apr 4;28(7):3082-94. doi: 10.1021/bi00433a052.
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The interaction of thrombin with fibrinogen. A structural basis for its specificity.
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Changes in interactions in complexes of hirudin derivatives and human alpha-thrombin due to different crystal forms.由于不同晶体形式导致的水蛭素衍生物与人α-凝血酶复合物中相互作用的变化。
Protein Sci. 1993 Oct;2(10):1630-42. doi: 10.1002/pro.5560021009.
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Structure of the Ser195Ala mutant of human alpha--thrombin complexed with fibrinopeptide A(7--16): evidence for residual catalytic activity.与纤维蛋白肽A(7-16)复合的人α-凝血酶Ser195Ala突变体的结构:残余催化活性的证据
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本文引用的文献

1
Structure of a bovine thrombin-hirudin51-65 complex determined by a combination of molecular replacement and graphics. Incorporation of known structural information in molecular replacement.通过分子置换与图形学相结合确定的牛凝血酶-水蛭素51-65复合物的结构。在分子置换中纳入已知结构信息。
Acta Crystallogr D Biol Crystallogr. 1996 May 1;52(Pt 3):453-64. doi: 10.1107/S0907444996000364.
2
Bovine thrombin complexed with an uncleavable analog of residues 7-19 of fibrinogen A alpha: geometry of the catalytic triad and interactions of the P1', P2', and P3' substrate residues.与纤维蛋白原Aα亚基7-19位残基不可裂解类似物复合的牛凝血酶:催化三联体的几何结构以及P1'、P2'和P3'底物残基的相互作用
Biochemistry. 1996 Oct 8;35(40):13030-9. doi: 10.1021/bi960656y.
3
The fibrinogen sequences that interact with thrombin.与凝血酶相互作用的纤维蛋白原序列。
Blood. 1993 Jun 15;81(12):3186-92.
4
A player of many parts: the spotlight falls on thrombin's structure.身兼多职的角色:聚焦凝血酶的结构
Thromb Res. 1993 Jan 1;69(1):1-58. doi: 10.1016/0049-3848(93)90002-6.
5
Mechanism of action of thrombin on fibrinogen. Direct evidence for the involvement of phenylalanine at position P9.凝血酶对纤维蛋白原的作用机制。P9位苯丙氨酸参与作用的直接证据。
Biochemistry. 1982 Nov 23;21(24):6167-71. doi: 10.1021/bi00267a022.
6
Mechanism of action of thrombin on fibrinogen. Kinetic evidence for involvement of aspartic acid at position P10.凝血酶对纤维蛋白原的作用机制。P10位天冬氨酸参与作用的动力学证据。
Biochemistry. 1983 Aug 30;22(18):4170-4. doi: 10.1021/bi00287a002.
7
Covalent structure of fibrinogen.纤维蛋白原的共价结构。
Ann N Y Acad Sci. 1983 Jun 27;408:28-43. doi: 10.1111/j.1749-6632.1983.tb23232.x.
8
Hydrogen bonding in globular proteins.球状蛋白质中的氢键。
Prog Biophys Mol Biol. 1984;44(2):97-179. doi: 10.1016/0079-6107(84)90007-5.
9
On the size of the active site in proteases. I. Papain.关于蛋白酶活性位点的大小。I. 木瓜蛋白酶。
Biochem Biophys Res Commun. 1967 Apr 20;27(2):157-62. doi: 10.1016/s0006-291x(67)80055-x.
10
Fibrinogen Milano II: a congenital dysfibrinogenaemia associated with juvenile arterial and venous thrombosis.纤维蛋白原米兰II型:一种与青少年动静脉血栓形成相关的先天性异常纤维蛋白原血症。
Thromb Haemost. 1986 Feb 28;55(1):131-5.

与牛凝血酶结合的纤维蛋白原-Aα肽1-23(F8Y)的晶体结构解释了为什么苯丙氨酸8突变为酪氨酸会强烈抑制精氨酸16处的正常切割。

Crystal structure of fibrinogen-Aalpha peptide 1-23 (F8Y) bound to bovine thrombin explains why the mutation of Phe-8 to tyrosine strongly inhibits normal cleavage at Arg-16.

作者信息

Malkowski M G, Martin P D, Lord S T, Edwards B F

机构信息

Department of Biochemistry, Wayne State University, 540 E. Canfield Avenue, Detroit, MI 48201, USA.

出版信息

Biochem J. 1997 Sep 15;326 ( Pt 3)(Pt 3):815-22. doi: 10.1042/bj3260815.

DOI:10.1042/bj3260815
PMID:9307032
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1218737/
Abstract

A peptide containing residues 1-50 of the Aalpha-chain of fibrinogen, expressed as a fusion peptide with beta-galactosidase, is rapidly cleaved by thrombin at Arg-16, similarly to whole fibrinogen. When Phe-8, which is highly conserved, is replaced with tyrosine (F8Y), the cleavage is slowed drastically [Lord, Byrd, Hede, Wei and Colby (1990) J. Biol. Chem. 265, 838-843]. To examine the structural basis for this result, we have determined the crystal structure of bovine thrombin complexed with a synthetic peptide containing residues 1-23 of fibrinogen Aalpha and the F8Y mutation. The crystals are in space group P43212, with unit-cell dimensions of a = 88.3 A (1 A = 0.1 nm), c = 195.5 A and two complexes in the asymmetric unit. The final R factor is 0.183 for 2sigma data from 7.0 to 2.5 A resolution. There is continuous density for the five residues in the P3, P2, P1, P1' and P2' positions of the peptide (Gly-14f to Pro-18f) at the active site of thrombin, and isolated but well-defined density for Tyr-8f at position P9 in the hydrophobic pocket of thrombin. The tyrosine residue is shifted relative to phenylalanine in the native peptide because the phenol side chain is larger and makes a novel, intrapeptide hydrogen bond with Gly-14f. Adjacent peptide residues cannot form the hydrogen bonds that stabilize the secondary structure of the native peptide. Consequently, the 'reaction'geometry at the scissile bond, eight residues from the mutation, is perturbed and the peptide is mostly uncleaved in the crystal structure.

摘要

一种包含纤维蛋白原Aα链1 - 50位残基的肽,以与β - 半乳糖苷酶融合肽的形式表达,与完整纤维蛋白原类似,在精氨酸 - 16处被凝血酶快速切割。当高度保守的苯丙氨酸 - 8被酪氨酸取代(F8Y)时,切割速度大幅减慢[洛德、伯德、赫德、魏和科尔比(1990年)《生物化学杂志》265卷,838 - 843页]。为研究此结果的结构基础,我们测定了与含纤维蛋白原Aα链1 - 23位残基及F8Y突变的合成肽复合的牛凝血酶的晶体结构。晶体属于空间群P43212,晶胞参数a = 88.3 Å(1 Å = 0.1 nm),c = 195.5 Å,不对称单元中有两个复合物。对于分辨率为7.0至2.5 Å的2σ数据,最终R因子为0.183。在凝血酶活性位点处,肽的P3、P2、P1、P1'和P2'位置的五个残基(甘氨酸 - 14f至脯氨酸 - 18f)有连续电子密度,在凝血酶疏水口袋的P9位置,酪氨酸 - 8f有孤立但清晰定义的电子密度。酪氨酸残基相对于天然肽中的苯丙氨酸发生了位移,因为酚侧链更大,并与甘氨酸 - 14f形成了新的肽内氢键。相邻肽残基无法形成稳定天然肽二级结构的氢键。因此,距突变位点八个残基处的可裂解键的“反应”几何结构受到干扰,在晶体结构中该肽大多未被切割。