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一种假定的与小鼠Xlr(X连锁,淋巴细胞调节)蛋白等效的人类蛋白。

A putative human equivalent of the murine Xlr (X-linked, lymphocyte-regulated) protein.

作者信息

Allenet B, Escalier D, Garchon H J

机构信息

INSERM U25, Hôpital Necker, Paris, France.

出版信息

Mamm Genome. 1995 Sep;6(9):640-4. doi: 10.1007/BF00352372.

Abstract

The murine Xlr (X-linked, lymphocyte-regulated) gene family was originally identified by subtractive cDNA hybridization and cloning. It was found to encode two 30-kDa nuclear proteins expressed in lymphoid cells and in primary spermatocytes in a developmentally regulated manner. Our data show that, in contrast to most X-linked genes, the Xlr family is not conserved at the DNA level between mouse and human. However, using anti-Xlr antibodies, an Xlr-immunoreactive nuclear protein of M(r) 30,000 was characterized in human RAJI B-lymphoblastoid cells by flow cytofluorimetry, by immunoblotting, and by immunocytolabeling. An Xlr-like molecule was also found to be expressed in human activated lymphocytes and in human primary spermatocytes, with a stage specificity similar to that known in the mouse. In contrast, no Xlr-immunoreactive protein was detected in a series of human tissues including brain, skeletal muscle, colon, liver, and kidney, revealing a tissue-specific expression pattern similar to that of murine Xlr. These findings most likely identify a human equivalent of Xlr. The Xlr genes belong to a small category of X-linked genes, including STS, MIC2, CSF2RA, and KAL, that diverge at the DNA level in human and in mice. Characterization of the human XLR gene(s) should now be feasible with anti-Xlr antibodies and an expression cloning system. It should provide new insights into the evolution of mammalian X Chromosome (Chr).

摘要

小鼠Xlr(X连锁、淋巴细胞调节)基因家族最初是通过消减cDNA杂交和克隆鉴定出来的。发现它编码两种30 kDa的核蛋白,以发育调节的方式在淋巴细胞和初级精母细胞中表达。我们的数据表明,与大多数X连锁基因不同,Xlr家族在小鼠和人类之间的DNA水平上并不保守。然而,使用抗Xlr抗体,通过流式细胞荧光术、免疫印迹和免疫细胞标记,在人RAJI B淋巴母细胞中鉴定出一种分子量为30,000的Xlr免疫反应性核蛋白。还发现一种Xlr样分子在人活化淋巴细胞和人初级精母细胞中表达,其阶段特异性与小鼠中已知的相似。相比之下,在包括脑、骨骼肌、结肠、肝和肾在内一系列人类组织中未检测到Xlr免疫反应性蛋白,揭示出与小鼠Xlr相似的组织特异性表达模式。这些发现很可能鉴定出了Xlr的人类同源物。Xlr基因属于一小类X连锁基因,包括STS、MIC2、CSF2RA和KAL,它们在人类和小鼠的DNA水平上存在差异(分歧)。现在利用抗Xlr抗体和表达克隆系统对人类XLR基因进行表征应该是可行的。这应该能为哺乳动物X染色体(Chr)的进化提供新的见解。

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