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人类Pim-1激酶组成型活性的结构基础及独特的核苷酸结合模式

Structural basis of constitutive activity and a unique nucleotide binding mode of human Pim-1 kinase.

作者信息

Qian Kevin C, Wang Lian, Hickey Eugene R, Studts Joey, Barringer Kevin, Peng Charline, Kronkaitis Anthony, Li Jun, White Andre, Mische Sheenah, Farmer Bennett

机构信息

Departments of Medicinal Chemistry and Immunology and Inflammation, Boehringer Ingelheim Pharmaceuticals, Inc., Research and Development, 175 Briar Ridge Rd., Ridgefield, CT 06877, USA.

出版信息

J Biol Chem. 2005 Feb 18;280(7):6130-7. doi: 10.1074/jbc.M409123200. Epub 2004 Nov 3.

DOI:10.1074/jbc.M409123200
PMID:15525646
Abstract

Pim-1 kinase is a member of a distinct class of serine/threonine kinases consisting of Pim-1, Pim-2, and Pim-3. Pim kinases are highly homologous to one another and share a unique consensus hinge region sequence, ER-PXPX, with its two proline residues separated by a non-conserved residue, but they (Pim kinases) have <30% sequence identity with other kinases. Pim-1 has been implicated in both cytokine-induced signal transduction and the development of lymphoid malignancies. We have determined the crystal structures of apo Pim-1 kinase and its AMP-PNP (5'-adenylyl-beta,gamma-imidodiphosphate) complex to 2.1-angstroms resolutions. The structures reveal the following. 1) The kinase adopts a constitutively active conformation, and extensive hydrophobic and hydrogen bond interactions between the activation loop and the catalytic loop might be the structural basis for maintaining such a conformation. 2) The hinge region has a novel architecture and hydrogen-bonding pattern, which not only expand the ATP pocket but also serve to establish unambiguously the alignment of the Pim-1 hinge region with that of other kinases. 3) The binding mode of AMP-PNP to Pim-1 kinase is unique and does not involve a critical hinge region hydrogen bond interaction. Analysis of the reported Pim-1 kinase-domain structures leads to a hypothesis as to how Pim kinase activity might be regulated in vivo.

摘要

Pim-1激酶是由Pim-1、Pim-2和Pim-3组成的一类独特的丝氨酸/苏氨酸激酶成员。Pim激酶彼此高度同源,共享一个独特的共有铰链区序列ER-PXPX,其两个脯氨酸残基被一个非保守残基隔开,但它们(Pim激酶)与其他激酶的序列同一性小于30%。Pim-1已被证明与细胞因子诱导的信号转导以及淋巴恶性肿瘤的发展有关。我们已经确定了无配体Pim-1激酶及其AMP-PNP(5'-腺苷-β,γ-亚氨基二磷酸)复合物的晶体结构,分辨率达到2.1埃。这些结构揭示了以下几点。1)该激酶采用组成型活性构象,激活环与催化环之间广泛的疏水和氢键相互作用可能是维持这种构象的结构基础。2)铰链区具有新颖的结构和氢键模式,不仅扩大了ATP口袋,还明确地确定了Pim-1铰链区与其他激酶铰链区的对齐方式。3)AMP-PNP与Pim-1激酶的结合模式独特,不涉及关键的铰链区氢键相互作用。对已报道的Pim-1激酶结构域结构的分析得出了一个关于Pim激酶活性在体内可能如何被调节的假设。

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