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活性人子宫组织纤溶酶原激活剂在酵母中的表达。

Expression of active human uterine tissue plasminogen activator in yeast.

作者信息

Lemontt J F, Wei C M, Dackowski W R

出版信息

DNA. 1985 Dec;4(6):419-28. doi: 10.1089/dna.1985.4.419.

Abstract

Tissue-type plasminogen activator (tPA) cDNA derived from human uterine mRNA was inserted into different yeast expression vectors. All such expression plasmids carried a yeast acid phosphatase (PHO5) promoter, a 2-micron plasmid replication origin, transcription termination signals, and a selectable TRP1 gene. Plasmid pYBDT-10 contained the entire tPA coding region ("pre-pro-tPA"), pYBDT-10-PRO contained a sequence encoding the putative pro-tPA precusor, and pYBDT-6 contained only a mature tPA cDNA fused precisely in frame to the sequence encoding the entire signal peptide of acid phosphatase. All constructions directed the synthesis of single-chain tPA proteins that were readily precipitated with a specific antibody directed against human uterine tPA. Electrophoretic mobilities were approximately the same as those of the Bowes melanoma single-chain tPA and a 68-kD protein marker. Treatment of immunoprecipitates with endoglycosidase H resulted in increased electrophoretic mobilities, suggesting that these yeast products are glycosylated. Despite the use of either human or yeast signal sequences, however, tPA produced in yeast was not secreted into the culture medium, but rather was found only in cells following disruption with glass beads. Although this cellular tPA exhibited fibrinolytic activity, most of the activity was associated with large cellular debris.

摘要

将源自人子宫mRNA的组织型纤溶酶原激活剂(tPA)cDNA插入不同的酵母表达载体中。所有这些表达质粒都带有酵母酸性磷酸酶(PHO5)启动子、2微米质粒复制起点、转录终止信号和一个可选的TRP1基因。质粒pYBDT - 10含有完整的tPA编码区(“前 - 原 - tPA”),pYBDT - 10 - PRO含有编码假定的原 - tPA前体的序列,pYBDT - 6仅含有与酸性磷酸酶整个信号肽编码序列精确框内融合的成熟tPA cDNA。所有构建体都指导合成单链tPA蛋白,这些蛋白很容易被针对人子宫tPA的特异性抗体沉淀。电泳迁移率与鲍伊斯黑色素瘤单链tPA和68-kD蛋白标志物的迁移率大致相同。用内切糖苷酶H处理免疫沉淀物导致电泳迁移率增加,表明这些酵母产物是糖基化的。然而,尽管使用了人或酵母信号序列,酵母中产生的tPA并未分泌到培养基中,而是仅在玻璃珠破碎细胞后才在细胞中发现。尽管这种细胞内的tPA表现出纤维蛋白溶解活性,但大部分活性与大的细胞碎片相关。

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