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胆固醇14-甲基十六烷酸酯对肽链延伸所需的某些核糖体功能的影响。

Influence of cholesteryl 14-methylhexadecanoate on some ribosomal functions required for peptide elongation.

作者信息

Hradec J, Dusek Z, Mach O

出版信息

Biochem J. 1974 Feb;138(2):147-54. doi: 10.1042/bj1380147.

Abstract
  1. Polyribosomes and ribosomal subunits from rat liver were adsorbed on a cellulosic ion-exchange adsorbent, freeze-dried and extracted with organic solvents. The activity of extracted particles in peptide elongation was tested in the presence of purified peptideelongation factors. 2. Chloroform-methanol mixture (2:1, v/v) extracted 1.87+/-0.15 pmol of cholesteryl 14-methylhexadecanoate/pmol of the smaller ribosomal subunit and 0.92+/-0.11 pmol/pmol of the larger subunit. 3. In the presence of transferase I, extracted polyribosomes and 40S subunits bound more phenylalanyl-tRNA than did control non-extracted particles. The same binding as in control mixtures was obtained with extracted particles supplemented with cholesteryl 14-methylhexadecanoate in quantities corresponding to those extracted. 4. The polymerization of phenylalanine was greatly decreased with extracted polyribosomes and subunits and addition of the cholesteryl ester could not fully restore the original activity. 5. Extraction significantly decreased the activity of the P site of peptidyl transferase and normal activity was recovered after the addition of the ester. The A site of peptidyl transferase in extracted polyribosomes showed an increased activity when compared with non-extracted polyribosomes. 6. Cholesteryl 14-methylhexadecanoate apparently affects the function of the ribosomal A site and peptidyl transferase site and probably also that of the guanosine triphosphatase site and P site. The presence of different amounts of the ester in polyribosomes may be one of the mechanisms modulating peptide elongation at the ribosomal level.
摘要
  1. 大鼠肝脏的多核糖体和核糖体亚基吸附在纤维素离子交换吸附剂上,冻干后用有机溶剂萃取。在纯化的肽延伸因子存在的情况下,测试萃取颗粒在肽延伸中的活性。2. 氯仿 - 甲醇混合物(2:1,v/v)从小核糖体亚基中每皮摩尔萃取1.87±0.15皮摩尔的14 - 甲基十六烷酸胆固醇酯,从大核糖体亚基中每皮摩尔萃取0.92±0.11皮摩尔。3. 在转移酶I存在的情况下,萃取的多核糖体和40S亚基比未萃取的对照颗粒结合更多的苯丙氨酰 - tRNA。用补充了与萃取量相当的14 - 甲基十六烷酸胆固醇酯的萃取颗粒,可获得与对照混合物相同的结合效果。4. 萃取的多核糖体和亚基使苯丙氨酸的聚合反应大大降低,添加胆固醇酯不能完全恢复其原始活性。5. 萃取显著降低了肽基转移酶P位点的活性,添加酯后恢复了正常活性。与未萃取的多核糖体相比,萃取的多核糖体中肽基转移酶的A位点活性增加。6. 14 - 甲基十六烷酸胆固醇酯显然影响核糖体A位点和肽基转移酶位点的功能,可能还影响鸟苷三磷酸酶位点和P位点的功能。多核糖体中不同量酯的存在可能是在核糖体水平调节肽延伸的机制之一。

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