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100 kDa Ras 鸟苷三磷酸酶激活蛋白的物种特异性及器官、细胞和亚细胞定位

Species specificity and organ, cellular and subcellular localization of the 100 kDa Ras GTPase activating protein.

作者信息

Mollat P, Fournier A, Yang C Z, Alsat E, Zhang Y, Evain-Brion D, Grassi J, Thang M N

机构信息

Unité 245 INSERM, Hôpital Saint-Antoine, Paris, France.

出版信息

J Cell Sci. 1994 Mar;107 ( Pt 3):427-35. doi: 10.1242/jcs.107.3.427.

Abstract

A p100-GAP isoform, generated by an alternative splicing mechanism that eliminates the 180 hydrophobic amino acids at the amino terminus of p120-GAP, has been described in human placenta, in addition to the known p120GAP and neurofibromin. This p100-GAP possesses full Ras-GTPase stimulating activity. p120-GAP is ubiquitously localized in the cytosol while the localization of p100-GAP is unknown. Here we have explored the precise localization of p100-GAP and show that p100-GAP is present only in extracts of primate placenta. It is abundant in both human and Maccaca Rhesus placentae, where it is present in far larger amounts than p120-GAP. The p100-GAP is species-specific since it was not detected in the placenta of pig, sheep, mouse or rat. p100-GAP was also found to be organ-specific, since it was not detectable in organs other than the placenta. In this connection, we substantiated our previous finding that p100-GAP is mainly localized in the trophoblasts. Both subcellular trophoblast fractionation and immunofluorescence analyses showed that this protein was distributed between the cytosol, plasma membrane and a fraction bound to the nucleus, but not inside it. This highly restrictive specificity of p100-GAP localization in relation to species, organ and cell type, confirms the extreme singularity of this protein, and strongly suggests a particular specific function in the trophoblast.

摘要

除了已知的p120-GAP和神经纤维瘤蛋白外,在人胎盘中还发现了一种p100-GAP同工型,它是通过选择性剪接机制产生的,该机制去除了p120-GAP氨基末端的180个疏水氨基酸。这种p100-GAP具有完整的Ras-GTPase刺激活性。p120-GAP普遍定位于细胞质中,而p100-GAP的定位尚不清楚。在这里,我们探索了p100-GAP的精确定位,并表明p100-GAP仅存在于灵长类胎盘提取物中。它在人类和恒河猴胎盘中都很丰富,其含量远高于p120-GAP。p100-GAP具有物种特异性,因为在猪、羊、小鼠或大鼠的胎盘中未检测到。p100-GAP还具有器官特异性,因为在胎盘以外的器官中无法检测到。在这方面,我们证实了之前的发现,即p100-GAP主要定位于滋养层细胞。滋养层细胞亚细胞分级分离和免疫荧光分析均表明,该蛋白分布于细胞质、质膜和与细胞核结合的部分,但不在细胞核内。p100-GAP在物种、器官和细胞类型方面具有高度限制性的特异性,证实了该蛋白的极端独特性,并强烈暗示其在滋养层细胞中具有特定的功能。

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