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利用免疫细胞化学和原位杂交技术在培养的肝癌Hep G2细胞中进行α-胰蛋白酶抑制剂及其不同mRNA的光镜检测。

Light microscopical detection of inter-alpha-trypsin inhibitor and its different mRNAs in cultured hepatoma Hep G2 cells using immunocytochemical and in situ hybridization techniques.

作者信息

Borghi H, Callé A, Sesboüé R, Bourguignon J, Diarra-Mehrpour M, Martin J P

机构信息

Unité de Recherche de Physiologie et Génétique Rénale et Pulmonaire, INSERM U 295, Faculté de Médecine et de Pharmacie de Rouen, St Etienne Rouvray, France.

出版信息

Histochem J. 1994 Mar;26(3):252-61.

PMID:7515868
Abstract

The Hep G2 hepatoma cell line synthesizes the inter-alpha-trypsin inhibitor (ITI). This protease inhibitor and the other proteins of this family include four polypeptides chains: three heavy chains (HC1, HC2, HC3) and one light chain (bikunin). In the present study, we have demonstrated by immunofluorescence that ITI is detected mainly in perinuclear cytoplasmic zones comparable to those of albumin or alpha-1-antitrypsin. The presence of the mRNAs of the four polypeptide chains in all Hep G2 cells of a non-synchronized culture have been demonstrated by in situ hybridization. An evaluation of the transcription of the four ITI genes through an analysis of markings brings to the fore a clearly much higher rate of mRNAs from the light chain than from the heavy chains. The mRNAs corresponding to the HC2 chains are more heavily represented than are those corresponding to the HC1 and HC3 chains. In Hep G2 cells in culture, a quantification of mRNAs based on the in situ hybridization technique shows that their relative quantities, in decreasing order, are those of L, HC2, HC3 and HC1.

摘要

Hep G2肝癌细胞系可合成α-胰蛋白酶抑制剂(ITI)。这种蛋白酶抑制剂以及该家族的其他蛋白质包含四条多肽链:三条重链(HC1、HC2、HC3)和一条轻链(抑酶肽)。在本研究中,我们通过免疫荧光证明,ITI主要在与白蛋白或α-1抗胰蛋白酶相似的核周细胞质区域被检测到。通过原位杂交已证明,在非同步培养的所有Hep G2细胞中均存在四条多肽链的mRNA。通过标记分析对四个ITI基因的转录进行评估,结果表明轻链mRNA的转录率明显高于重链。与HC2链对应的mRNA比重于与HC1和HC3链对应的mRNA。在培养的Hep G2细胞中,基于原位杂交技术对mRNA进行定量分析表明,其相对含量从高到低依次为L、HC2、HC3和HC1。

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