大麦类囊体叶绿素a/b结合蛋白单克隆抗体的体外翻译产物检测

G Høyer-Hansen, L S Hønberg, R Bassi
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引用次数: 3

摘要

大麦光系统I光收获蛋白(LHCI)的多肽具有某些共同的表位。如交叉反应的单克隆抗体所示,叶绿素a/b-蛋白1 (Chla/b-P1 = CP29)中至少有两个共同的表位存在(14)。这些抗体用于免疫鉴定在mrna依赖的无细胞兔网织细胞裂解液中翻译的多肽。单克隆抗体CMpLHCI:2仅从polyA+ RNA引物的体外翻译中提取一个分子量为28 kD的多肽。如果将该抗体与PSI-200混合后再加入到翻译中,则未发现28kd沉淀带。从12小时青大麦中分离的LHCI转录本的翻译能力远高于6小时青大麦。在类囊体膜中缺乏LHCI多肽的突变病毒-k23的polyA+ RNA中也发现了LHCI多肽的转录本。单克隆抗体CMpCh1a/b-P1:1从polyA+ RNA引物的体外翻译中沉淀分子量为31 kD的多肽。因此,当抗体与前体蛋白反应时,两种抗体与成熟蛋白表现出的交叉反应性并不存在。
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Probing in vitro translation products with monoclonal antibodies to chlorophyll a/b-binding proteins of barley thylakoids.

The polypeptides of the barley light-harvesting protein of photosystem I (LHCI) share certain epitopes. At least two of these common epitopes are present in chlorophyll a/b-protein 1 (Chla/b-P1 = CP29), as shown by cross-reacting monoclonal antibodies (14). These antibodies were employed for immunological identification of polypeptides translated in vitro in an mRNA-dependent cell-free rabbit reticulocyte lysate. The monoclonal antibody CMpLHCI:2 precipitated only one polypeptide of molecular weight 28 kD from in vitro translates primed with polyA+ RNA. No 28 kD precipitation band was found, if this antibody was mixed with a PSI-200 preparation before it was added to the translate. The translational capacity of the LHCI transcripts isolated from 12 hours greened barley was much higher than those isolated from 6 hours greened barley. Transcripts for LHCI polypeptides were also found among the polyA+ RNA of the mutant viridis-k23, which is devoid of LHCI polypeptides in its thylakoid membranes. The monoclonal antibody CMpCh1a/b-P1:1 precipitated a polypeptide of molecular weight 31 kD from in vitro translates primed with polyA+ RNA. Thus, the cross-reactivity the two antibodies show with the mature proteins is not found when the antibodies are reacted with the precursor proteins.

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