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对恶性转化的人类细胞系中赖氨酰氧化酶信使核糖核酸进行定量聚合酶链反应表明,它们的低赖氨酰氧化酶活性是由于其信使核糖核酸数量少以及相应基因的转录水平低所致。

Quantitative polymerase chain reaction of lysyl oxidase mRNA in malignantly transformed human cell lines demonstrates that their low lysyl oxidase activity is due to low quantities of its mRNA and low levels of transcription of the respective gene.

作者信息

Hämäläinen E R, Kemppainen R, Kuivaniemi H, Tromp G, Vaheri A, Pihlajaniemi T, Kivirikko K I

机构信息

Collagen Research Unit, University of Oulu, Finland.

出版信息

J Biol Chem. 1995 Sep 15;270(37):21590-3. doi: 10.1074/jbc.270.37.21590.

Abstract

Lysyl oxidase (EC 1.4.3.13), an extracellular copper amino oxidase, initiates the cross-linking of collagens and elastin by catalyzing oxidative deamination of the epsilon-amino group in certain lysine and hydroxylysine residues. We developed here a polymerase chain reaction (PCR) method for the quantification of lysyl oxidase mRNA in which a synthetic RNA is used as an internal standard for coamplification with the targeted mRNA. The amount of lysyl oxidase mRNA when studied by Northern blot analysis and the number of lysyl oxidase mRNA molecules when determined by the quantitative PCR method were found to be markedly low in various malignantly transformed cell lines relative to control cell lines, quantitative PCR indicating values of about 2-10% of those in the controls. No difference was found in the number of beta-actin mRNA molecules between the transformed cells and the controls. Nuclear runoff experiments indicated that most if not all of the decrease in the number of lysyl oxidase mRNA molecules can be explained by diminished transcription of the respective gene.

摘要

赖氨酰氧化酶(EC 1.4.3.13)是一种细胞外铜氨基氧化酶,通过催化某些赖氨酸和羟赖氨酸残基中ε-氨基的氧化脱氨作用,启动胶原蛋白和弹性蛋白的交联。我们在此开发了一种聚合酶链反应(PCR)方法,用于定量赖氨酰氧化酶mRNA,其中使用合成RNA作为内部标准与目标mRNA共同扩增。通过Northern印迹分析研究时,发现各种恶性转化细胞系中赖氨酰氧化酶mRNA的量,以及通过定量PCR方法测定时赖氨酰氧化酶mRNA分子的数量,相对于对照细胞系明显较低,定量PCR表明其值约为对照中的2-10%。转化细胞和对照之间β-肌动蛋白mRNA分子的数量没有差异。核转录实验表明,赖氨酰氧化酶mRNA分子数量的减少,即使不是全部,大部分也可以用相应基因转录的减少来解释。

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