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缺氧对内皮细胞3-磷酸甘油醛脱氢酶表达的调控

Regulation of endothelial cell glyceraldehyde-3-phosphate dehydrogenase expression by hypoxia.

作者信息

Graven K K, Troxler R F, Kornfeld H, Panchenko M V, Farber H W

机构信息

Pulmonary Center, Boston University School of Medicine, Massachusetts 02118.

出版信息

J Biol Chem. 1994 Sep 30;269(39):24446-53.

PMID:7929107
Abstract

Exposure of endothelial cells (EC) to hypoxia results in the increased expression of a distinct set of proteins with molecular masses of 56, 47, 39, 36, and 34 kDa. Their induction appears to be unique to EC and the stress of decreased oxygen tension. To understand the mechanism(s) and significance of the up-regulation of these proteins we have identified the 36-kDa protein by limited amino-terminal amino acid sequencing. The 21-amino acid sequence from the bovine protein exhibited 90.5% identity with the human sequence of the glycolytic enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH). Northern blot analysis showed that the time course and extent of EC GAPDH mRNA up-regulation correlated with the increase in 36-kDa protein synthesis. Nuclear runoff analysis demonstrated that this increase in GAPDH expression is regulated, in part, at the transcriptional level; however, the increase in the rate of transcription did not account for the entire mRNA accumulation, suggesting that GAPDH, like other hypoxia-regulated proteins, is posttranscriptionally regulated. Subcellular fractionation of hypoxic EC showed up-regulation of the 36-kDa protein in the cytoplasmic fraction and, to a lesser extent, in the nuclear fraction. The up-regulation of GAPDH in EC may be related to their relative hypoxia tolerance. Alternatively, the up-regulation of GAPDH in EC during hypoxia may be related to the potential nonglycolytic functions of this enzyme.

摘要

将内皮细胞(EC)暴露于低氧环境会导致一组分子量分别为56、47、39、36和34 kDa的独特蛋白质表达增加。它们的诱导似乎是内皮细胞特有的,且与氧张力降低的应激有关。为了了解这些蛋白质上调的机制和意义,我们通过有限的氨基末端氨基酸测序鉴定了36 kDa的蛋白质。牛蛋白的21个氨基酸序列与糖酵解酶甘油醛-3-磷酸脱氢酶(GAPDH)的人类序列具有90.5%的同源性。Northern印迹分析表明,内皮细胞GAPDH mRNA上调的时间进程和程度与36 kDa蛋白质合成的增加相关。核转录分析表明,GAPDH表达的这种增加部分是在转录水平上受到调控的;然而,转录速率的增加并不能解释整个mRNA的积累,这表明GAPDH与其他低氧调节蛋白一样,在转录后受到调控。对低氧内皮细胞进行亚细胞分级分离显示,36 kDa蛋白质在细胞质部分上调,在核部分上调程度较小。内皮细胞中GAPDH的上调可能与其相对的低氧耐受性有关。或者,低氧期间内皮细胞中GAPDH的上调可能与其该酶潜在的非糖酵解功能有关。

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