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Eh Klp5是驱动蛋白5家族的一个不同成员,它调节溶组织内阿米巴的基因组含量和微管组装。

Eh Klp5 is a divergent member of the kinesin 5 family that regulates genome content and microtubular assembly in Entamoeba histolytica.

作者信息

Dastidar Promita Ghosh, Majumder Shubhra, Lohia Anuradha

机构信息

Department of Biochemistry, Bose Institute, Kolkata 700054, India.

出版信息

Cell Microbiol. 2007 Feb;9(2):316-28. doi: 10.1111/j.1462-5822.2006.00788.x. Epub 2006 Aug 22.

DOI:10.1111/j.1462-5822.2006.00788.x
PMID:16925786
Abstract

Earlier studies have established two unusual features in the cell division cycle of Entamoeba histolytica. First, microtubules form a radial assembly instead of a bipolar mitotic spindle, and second, the genome content of E. histolytica cells varied from 1x to 6x or more. In this study, Eh Klp5 was identified as a divergent member of the BimC kinesin family that is known to regulate formation and stabilization of the mitotic spindle in other eukaryotes. In contrast to earlier studies, we show here that bipolar microtubular spindles were formed in E. histolytica but were visible only in 8-12% of the cells after treatment with taxol. The number of bipolar spindles was significantly increased in Eh Klp5 stable transformants (20-25%) whereas Eh Klp5 double-stranded RNA (dsRNA) transformants did not show any spindles (< 1%). The genome content of Eh Klp5 stable transformants was regulated between 1x and 2x unlike control cells. Binucleated cells accumulated in Eh Klp5 dsRNA transformants and after inhibition of Eh Klp5 with small molecule inhibitors in control cells, suggesting that cytokinesis was delayed in the absence of Eh Klp5. Taken together, our results indicate that Eh Klp5 regulates microtubular assembly, genome content and cell division in E. histolytica. Additionally, Eh Klp5 showed alterations in its drug-binding site compared with its human homologue, Hs Eg5 and this was reflected in its reduced sensitivity to Eg5 inhibitors - monastrol and HR22C16 analogues.

摘要

早期研究已确定溶组织内阿米巴细胞分裂周期有两个不同寻常的特征。其一,微管形成放射状结构而非双极有丝分裂纺锤体;其二,溶组织内阿米巴细胞的基因组含量从1倍体变化到6倍体或更多。在本研究中,Eh Klp5被鉴定为BimC驱动蛋白家族的一个不同成员,已知该家族在其他真核生物中调节有丝分裂纺锤体的形成和稳定。与早期研究不同,我们在此表明,在溶组织内阿米巴中形成了双极微管纺锤体,但在用紫杉醇处理后仅在8% - 12%的细胞中可见。在Eh Klp5稳定转化体中双极纺锤体的数量显著增加(20% - 25%),而Eh Klp5双链RNA(dsRNA)转化体未显示任何纺锤体(<1%)。与对照细胞不同,Eh Klp5稳定转化体的基因组含量在1倍体和2倍体之间受到调节。在Eh Klp5 dsRNA转化体中双核细胞积累,并且在对照细胞中用小分子抑制剂抑制Eh Klp5后也出现这种情况,这表明在没有Eh Klp5的情况下胞质分裂延迟。综上所述,我们的结果表明Eh Klp5在溶组织内阿米巴中调节微管组装、基因组含量和细胞分裂。此外,与人类同源物Hs Eg5相比,Eh Klp5的药物结合位点发生了改变,这反映在其对Eg5抑制剂——monastrol和HR22C16类似物的敏感性降低上。

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