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猪脂肪酶的表达及补体D活性

Expression and complement d activity of porcine adipsin.

作者信息

Miner J L, Hahn K J, Spurlock M E, Staten N R

机构信息

Monsanto Company, Lincoln, Nebraska 68583-0908, USA.

出版信息

Protein Expr Purif. 2001 Oct;23(1):14-21. doi: 10.1006/prep.2001.1482.

Abstract

To learn how signals from adipocytes might be involved in regulation of energy intake and storage, we have begun to characterize the porcine complement protein, adipsin. Adipsin was originally identified as a protein that is produced rather specifically by adipocytes, is secreted, and is nearly absent in several obese rodent models. We now report that porcine adipsin mRNA sequence is 74% identical to rat and predicts a protein that has 82 and 68% identity to human and rat forms, respectively. Porcine adipsin has none of the asparagine glycosylation consensus sites which make recombinant expression of mouse adipsin in Escherichia coli impractical. We present a method for engineering the porcine cDNA to facilitate expression by E. coli and provide a protocol for refolding and purifying porcine adipsin protein and for immunoassay. We have found that in addition to adipose tissue, adipsin mRNA is present in gut tissues. Coupled with the fact that adipsin is required for processing of complement C3a-desArg, and that C3a-desArg is a potent stimulant of fatty acid acylation in adipocytes, the production of adipsin in the gut may be related to a mechanism for adipocyte removal of lipid from chylomicrons.

摘要

为了了解脂肪细胞发出的信号如何参与能量摄入和储存的调节,我们已开始对猪补体蛋白——脂肪酶进行特性描述。脂肪酶最初被鉴定为一种由脂肪细胞特异性产生、分泌且在几种肥胖啮齿动物模型中几乎不存在的蛋白质。我们现在报告,猪脂肪酶mRNA序列与大鼠的序列有74%的同源性,预测的蛋白质与人类和大鼠的脂肪酶分别有82%和68%的同源性。猪脂肪酶没有天冬酰胺糖基化共有位点,这使得在大肠杆菌中重组表达小鼠脂肪酶不切实际。我们提出了一种改造猪cDNA以促进其在大肠杆菌中表达的方法,并提供了猪脂肪酶蛋白重折叠、纯化及免疫测定的方案。我们发现,除脂肪组织外,肠道组织中也存在脂肪酶mRNA。鉴于脂肪酶是补体C3a -去精氨酸加工所必需的,且C3a -去精氨酸是脂肪细胞中脂肪酸酰化的有效刺激物,肠道中脂肪酶的产生可能与脂肪细胞从乳糜微粒中清除脂质的机制有关。

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