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中心体功能障碍与联会复合体蛋白 TEX12 的体细胞表达有关。

Centrosome dysfunction associated with somatic expression of the synaptonemal complex protein TEX12.

机构信息

Howard Hughes Medical Institute, Department of Microbiology and Molecular Genetics, University of California, Davis, CA, 95616, USA.

Institute of Systems, Molecular and Integrative Biology, University of Liverpool, Liverpool, L69 7ZB, UK.

出版信息

Commun Biol. 2021 Dec 8;4(1):1371. doi: 10.1038/s42003-021-02887-4.

Abstract

The synaptonemal complex (SC) is a supramolecular protein scaffold that mediates chromosome synapsis and facilitates crossing over during meiosis. In mammals, SC proteins are generally assumed to have no other function. Here, we show that SC protein TEX12 also localises to centrosomes during meiosis independently of chromosome synapsis. In somatic cells, ectopically expressed TEX12 similarly localises to centrosomes, where it is associated with centrosome amplification, a pathology correlated with cancer development. Indeed, TEX12 is identified as a cancer-testis antigen and proliferation of some cancer cells is TEX12-dependent. Moreover, somatic expression of TEX12 is aberrantly activated via retinoic acid signalling, which is commonly disregulated in cancer. Structure-function analysis reveals that phosphorylation of TEX12 on tyrosine 48 is important for centrosome amplification but not for recruitment of TEX12 to centrosomes. We conclude that TEX12 normally localises to meiotic centrosomes, but its misexpression in somatic cells can contribute to pathological amplification and dysfunction of centrosomes in cancers.

摘要

联会复合体(SC)是一种介导染色体联会并促进减数分裂中交叉的超分子蛋白质支架。在哺乳动物中,普遍认为 SC 蛋白没有其他功能。在这里,我们表明,SC 蛋白 TEX12 在减数分裂期间也独立于染色体联会而定位到中心体。在体细胞中,异位表达的 TEX12 也类似地定位到中心体,在那里它与中心体扩增相关,中心体扩增与癌症发展相关。事实上,TEX12 被鉴定为一种癌症-睾丸抗原,一些癌细胞的增殖依赖于 TEX12。此外,通过视黄酸信号转导异常激活体细胞表达 TEX12,而视黄酸信号转导在癌症中通常失调。结构-功能分析表明,TEX12 上酪氨酸 48 的磷酸化对于中心体扩增很重要,但对于 TEX12 招募到中心体则不重要。我们得出结论,TEX12 通常定位在减数分裂中心体中,但在体细胞中的异常表达可能导致癌症中心体病理性扩增和功能障碍。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/78af/8654964/673e8b0b3364/42003_2021_2887_Fig1_HTML.jpg

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