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通过与在大肠杆菌中产生的c-myc蛋白发生反应的单克隆抗体检测到的人类细胞中细胞分子的多样性。

Diversity of cellular molecules in human cells detected by monoclonal antibodies reactive with c-myc proteins produced in Escherichia coli.

作者信息

Naoe T, Nozaki N, Yamada K, Okazaki T, Nakayama E, Kurosawa Y, Shiku H

机构信息

Department of Internal Medicine, Nagoya University Branch Hospital.

出版信息

Jpn J Cancer Res. 1989 Aug;80(8):747-53. doi: 10.1111/j.1349-7006.1989.tb01709.x.

Abstract

Six clones of monoclonal antibodies, MYC-1 to -6, were prepared by using two kinds of truncated c-myc proteins, p23 and p42, produced in Escherichia coli as immunogens. Analysis with enzyme-linked immunosorbent assays and immunoblotting assays with peptides produced in Escherichia coli showed that 5 clones of monoclonal antibodies, MYC-1 to -4 and -6, were reactive with c-myc protein encoded by exon 2. The remaining one clone, MYC-5, was reactive with the portion of c-myc protein encoded by exon 3. All monoclonal antibodies were also reactive with phosphorylated c-myc protein produced by insect cells infected by the baculovirus expression vector with the human c-myc gene. With immunoblotting assays using cellular lysates, MYC-1 and -3 detected bands at the levels of 58 kDa and 60 kDa, MYC-5 detected a band at 56 kDa and MYC-6 detected bands at 68 kDa and 75 kDa. All of these bands were detectable in nuclear extracts of HL-60 and Colo320, both of which have amplified c-myc genes, and also the extract of RmycYl which is the c-myc gene transfectant into 3Yl rat cells. None of them was detectable in peripheral blood mononuclear cells and 3Yl, both of which lacked activated c-myc genes. This indicates that these nuclear proteins are either c-myc gene products or molecules closely related to the c-myc gene. The remaining two clones, MYC-2 and -4, detected a band at the level of 85 kDa in cytoplasmic extracts of all the above-mentioned cells independent of the presence of the c-myc gene. This suggests that 85 kDa protein might be irrelevant to the c-myc gene. The 56 kDa protein was detectable by MYC-5 in phytohemagglutinin-stimulated peripheral blood mononuclear cells as well as leukemic cells of some patients.

摘要

利用在大肠杆菌中产生的两种截短型c-myc蛋白p23和p42作为免疫原,制备了6个单克隆抗体克隆,即MYC-1至-6。通过酶联免疫吸附测定以及对在大肠杆菌中产生的肽进行免疫印迹分析表明,5个单克隆抗体克隆,即MYC-1至-4和-6,可与外显子2编码的c-myc蛋白发生反应。其余一个克隆MYC-5可与外显子3编码的c-myc蛋白部分发生反应。所有单克隆抗体也可与被携带人c-myc基因的杆状病毒表达载体感染的昆虫细胞产生的磷酸化c-myc蛋白发生反应。使用细胞裂解物进行免疫印迹分析时,MYC-1和-3在58 kDa和60 kDa水平检测到条带,MYC-5在56 kDa处检测到一条带,MYC-6在68 kDa和75 kDa处检测到条带。所有这些条带在HL-60和Colo320的核提取物中均可检测到,这两种细胞均扩增了c-myc基因,在转染了c-myc基因的3Yl大鼠细胞RmycYl的提取物中也可检测到。在缺乏活化c-myc基因的外周血单核细胞和3Yl中均未检测到这些条带。这表明这些核蛋白要么是c-myc基因产物,要么是与c-myc基因密切相关的分子。其余两个克隆MYC-2和-4在上述所有细胞的细胞质提取物中均在85 kDa水平检测到一条带,与c-myc基因的存在无关。这表明85 kDa蛋白可能与c-myc基因无关。MYC-5在植物血凝素刺激的外周血单核细胞以及一些患者的白血病细胞中可检测到56 kDa蛋白。

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本文引用的文献

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