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来自大肠杆菌诱导培养物的多核糖体在体外合成色氨酸酶。

Biosynthesis in vitro of tryptophanase by polyribosomes from induced cultures of Escherichia coli.

作者信息

Bashar S A, Parish J H, Brown M

出版信息

Biochem J. 1971 Jul;123(3):355-65. doi: 10.1042/bj1230355.

Abstract
  1. Polyribosomes were isolated from Escherichia coli grown in media in which tryptophanase is induced and in which it is repressed. The polyribosomes from the induced bacteria had a small amount of tryptophanase activity associated with them. 2. A portion of the enzyme activity remained bound to polyribosomes during centrifuging in sucrose gradients. 3. Incubation of tryptophanase-containing polyribosomes with puromycin released enzyme activity. 4. The binding of the enzyme to the polyribosomes did not depend on the presence of DNA. 5. When the polyribosomes were incubated under conditions of protein synthesis with supernatant fraction obtained from repressed bacteria, a small but statistically significant increase in enzyme activity was produced. 6. When a radioactive amino acid was included in the incubation mixture for the tryptophanase system a radioactive protein was obtained whose chromatographic, electrophoretic and sedimentation properties were identical with those of tryptophanase. 7. The amount of incorporation was consistent with the amount of new enzyme synthesis predicted by the increase in enzyme activity. Both radioactive incorporation and increase in enzyme activity were shown to be energy-dependent and also negative controls were obtained by using zero-time incubations or polyribosomes isolated from either repressed cells or a mutant lacking the ability to produce tryptophanase. 8. The distribution of radioactive leucine in the carboxyl region of the newly labelled tryptophanase was examined by digesting the labelled protein with carboxypeptidases. It was shown that the radioactivity was more highly concentrated towards the carboxyl terminus when the incubation times for protein synthesis were shorter (implying that, with longer incubation times, longer lengths of polypeptide chain contained radioactive amino acid residues).
摘要
  1. 从在诱导色氨酸酶的培养基以及抑制色氨酸酶的培养基中生长的大肠杆菌中分离出多核糖体。来自诱导细菌的多核糖体有少量与之相关的色氨酸酶活性。2. 在蔗糖梯度离心中,一部分酶活性仍与多核糖体结合。3. 含色氨酸酶的多核糖体与嘌呤霉素一起温育会释放出酶活性。4. 酶与多核糖体的结合不依赖于DNA的存在。5. 当多核糖体在蛋白质合成条件下与从抑制细菌中获得的上清液部分一起温育时,酶活性产生了虽小但具有统计学意义的增加。6. 当在色氨酸酶系统的温育混合物中加入放射性氨基酸时,获得了一种放射性蛋白质,其色谱、电泳和沉降特性与色氨酸酶相同。7. 掺入量与酶活性增加所预测的新酶合成量一致。放射性掺入和酶活性增加均显示为能量依赖性,并且通过使用零时间温育或从抑制细胞或缺乏产生色氨酸酶能力的突变体中分离的多核糖体获得了阴性对照。8. 通过用羧肽酶消化标记蛋白质,检查了新标记的色氨酸酶羧基区域中放射性亮氨酸的分布。结果表明,当蛋白质合成的温育时间较短时,放射性更高度集中在羧基末端(这意味着,温育时间越长,多肽链中含有放射性氨基酸残基的长度越长)。

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