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本文引用的文献

1
A mammalian peptidase specific for the hydrolysis of N-terminal alpha-L-glutamyl and aspartyl residues.一种特异性水解N端α-L-谷氨酰基和天冬氨酰基残基的哺乳动物肽酶。
Nature. 1962 Jun 2;194:867. doi: 10.1038/194867a0.
2
A tyrosine residue essential for catalytic activity in aminopeptidase A.氨肽酶A催化活性所必需的一个酪氨酸残基。
Biochem J. 1997 Nov 1;327 ( Pt 3)(Pt 3):883-9. doi: 10.1042/bj3270883.
3
Aminopeptidase A: distribution in rat brain nuclei and increased activity in spontaneously hypertensive rats.
Neuroscience. 1997 Jun;78(4):1187-93. doi: 10.1016/s0306-4522(96)00660-4.
4
Aminopeptidase B from the rat testis is a bifunctional enzyme structurally related to leukotriene-A4 hydrolase.来自大鼠睾丸的氨肽酶B是一种与白三烯-A4水解酶结构相关的双功能酶。
Proc Natl Acad Sci U S A. 1997 Apr 1;94(7):2963-8. doi: 10.1073/pnas.94.7.2963.
5
Proteolytic fragmentation reveals the oligomeric and domain structure of porcine aminopeptidase A.蛋白水解片段化揭示了猪氨肽酶A的寡聚体和结构域结构。
Biochemistry. 1997 Mar 11;36(10):3000-7. doi: 10.1021/bi962401q.
6
Molecular cloning and expression of rat liver aminopeptidase B.大鼠肝脏氨肽酶B的分子克隆与表达
J Biol Chem. 1996 Nov 29;271(48):30731-5. doi: 10.1074/jbc.271.48.30731.
7
Identification of metabolic pathways of brain angiotensin II and III using specific aminopeptidase inhibitors: predominant role of angiotensin III in the control of vasopressin release.使用特定氨肽酶抑制剂鉴定脑内血管紧张素II和III的代谢途径:血管紧张素III在控制血管加压素释放中的主要作用
Proc Natl Acad Sci U S A. 1996 Oct 15;93(21):11968-73. doi: 10.1073/pnas.93.21.11968.
8
Rat endothelin-converting enzyme-1 forms a dimer through Cys412 with a similar catalytic mechanism and a distinct substrate binding mechanism compared with neutral endopeptidase-24.11.大鼠内皮素转化酶-1通过半胱氨酸412形成二聚体,与中性内肽酶-24.11相比,其催化机制相似,但底物结合机制不同。
Biochem J. 1996 May 1;315 ( Pt 3)(Pt 3):863-7. doi: 10.1042/bj3150863.
9
Identification of glutamate residues essential for catalytic activity and zinc coordination in aminopeptidase A.鉴定氨肽酶A中催化活性和锌配位所必需的谷氨酸残基。
J Biol Chem. 1996 Apr 12;271(15):9069-74. doi: 10.1074/jbc.271.15.9069.
10
Human placental leucine aminopeptidase/oxytocinase. A new member of type II membrane-spanning zinc metallopeptidase family.人胎盘亮氨酸氨肽酶/催产素酶。II型跨膜锌金属肽酶家族的一个新成员。
J Biol Chem. 1996 Jan 5;271(1):56-61. doi: 10.1074/jbc.271.1.56.

一个谷氨酸残基对氨肽酶A的外肽酶特异性有贡献。

A glutamate residue contributes to the exopeptidase specificity in aminopeptidase A.

作者信息

Vazeux G, Iturrioz X, Corvol P, Llorens-Cortes C

机构信息

INSERM Unité 36, Collège de France, 3 rue d'Ulm, 75005 Paris, France.

出版信息

Biochem J. 1998 Sep 1;334 ( Pt 2)(Pt 2):407-13. doi: 10.1042/bj3340407.

DOI:10.1042/bj3340407
PMID:9716499
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1219703/
Abstract

Aminopeptidase A (EC 3.4.11.7, APA) is a 130 kDa membrane-bound aminopeptidase that contains the consensus sequence HEXXH (385-389) found in the zinc metalloprotease family, the zincins. Sequence alignment of the mouse APA with other monozinc-aminopeptidases indicates the presence of a highly conserved glutamate residue (Glu352 in APA) found in the conserved motif GAMEN (349-353). In monozinc-aminopeptidases, the negative charge of the glutamate side-chain carboxylate may constitute the anionic binding site involved in the recognition of the free amino group of substrates or inhibitors. The functional role of Glu352 in APA was investigated by substituting this residue with an aspartate (Asp352), a glycine (Gly352), a glutamine (Gln352) or an arginine (Arg352) residue by site-directed mutagenesis. Kinetic studies showed that the Km values of the mutant enzymes were unaffected, whereas kcat values were decreased 10-250-fold, resulting in a 10-, 30- 260- and 400-fold reduction in cleavage efficiencies for the mutants Asp352, Gly352, Gln352 and Arg352 respectively. The inhibitory potency of two different classes of inhibitors, a thiol and a phosphonate compound, was significantly (P<0.05) decreased by 10- and 4-fold respectively in the mutated enzymes. Moreover, the inhibitory potency of angiotensin I, used as a competitor of the synthetic substrate alpha-l-glutamyl beta-naphthylamide, displayed a 4-fold reduction (P<0.01) in the mutated enzymes, whereas the Ki values of its N-acetyl derivative were unchanged. These data strongly suggest that Glu352 is involved in the catalytic process of APA and contributes to the exopeptidase activity of this enzyme through interaction with the N-terminal part of substrates or inhibitors.

摘要

氨肽酶A(EC 3.4.11.7,APA)是一种130 kDa的膜结合氨肽酶,含有锌金属蛋白酶家族(锌指蛋白)中发现的共有序列HEXXH(385 - 389)。小鼠APA与其他单锌氨肽酶的序列比对表明,在保守基序GAMEN(349 - 353)中存在一个高度保守的谷氨酸残基(APA中的Glu352)。在单锌氨肽酶中,谷氨酸侧链羧酸盐的负电荷可能构成参与识别底物或抑制剂游离氨基的阴离子结合位点。通过定点诱变将该残基替换为天冬氨酸(Asp352)、甘氨酸(Gly352)、谷氨酰胺(Gln352)或精氨酸(Arg352)残基,研究了Glu352在APA中的功能作用。动力学研究表明,突变酶的Km值未受影响,而kcat值降低了10 - 250倍,导致突变体Asp352、Gly352、Gln352和Arg352的切割效率分别降低了10倍、30倍、260倍和400倍。两类不同抑制剂(一种硫醇和一种膦酸盐化合物)的抑制效力在突变酶中分别显著(P<0.05)降低了10倍和4倍。此外,用作合成底物α - l - 谷氨酰 - β - 萘酰胺竞争剂的血管紧张素I的抑制效力在突变酶中降低了4倍(P<0.01),而其N - 乙酰衍生物的Ki值未变。这些数据强烈表明,Glu352参与了APA的催化过程,并通过与底物或抑制剂的N端部分相互作用,对该酶的外肽酶活性有贡献。