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乙醛酸循环体生物合成过程中苹果酸合酶的寡聚化

Oligomerization of malate synthase during glyoxysome biosynthesis.

作者信息

Kruse C, Kindl H

出版信息

Arch Biochem Biophys. 1983 Jun;223(2):629-38. doi: 10.1016/0003-9861(83)90627-6.

Abstract

The octameric malate synthase, found in glyoxysomes of plants, is synthesized as monomeric precursor in the cytoplasm. The precursor form does not possess a different subunit molecular weight than the mature organellar enzyme, but differs from the organellar protein by not oligomerizing and aggregating. This was shown by synthesis in a cell-free reticulocyte lysate system programmed with cucumber poly A+-mRNA followed by immunoprecipitation of the radiolabeled translation products. The precursor form of malate synthase was also detected in vivo in the cytosol of pulse-labeled cucumber cotyledons after immunoprecipitation of the radiolabeled polypeptide. At low salt concentrations, mature malate synthase can be converted into aggregated forms. However, the precursor form obtained either by in vitro translation or by extraction from the cytosol after short pulses of radioactive methionine, could neither be oligomerized into the octameric form nor aggregated into the 100-S form. Processing of malate synthase, assumed to be a requisite for oligomerization, took place rapidly in the glyoxysomes, but proceeded only slowly in the cytosol. This was demonstrated both by the uptake of in vitro-translated malate synthase into glyoxysomes, and by analysis of newly synthesized malate synthase detectable in glyoxysomes in vivo. In both cases the octamer was by far the predominant form.

摘要

在植物乙醛酸循环体中发现的八聚体苹果酸合酶,在细胞质中作为单体前体合成。前体形式与成熟的细胞器酶相比,亚基分子量并无差异,但与细胞器蛋白的不同之处在于它不会寡聚和聚集。在用黄瓜多聚腺苷酸加尾mRNA编程的无细胞网织红细胞裂解物系统中进行合成,随后对放射性标记的翻译产物进行免疫沉淀,结果证明了这一点。在对放射性标记的多肽进行免疫沉淀后,在脉冲标记的黄瓜子叶的细胞质中也在体内检测到了苹果酸合酶的前体形式。在低盐浓度下,成熟的苹果酸合酶可转化为聚集形式。然而,通过体外翻译或在短时间放射性甲硫氨酸脉冲后从细胞质中提取获得的前体形式,既不能寡聚成八聚体形式,也不能聚集成100-S形式。苹果酸合酶的加工过程,被认为是寡聚化的必要条件,在乙醛酸循环体中迅速发生,但在细胞质中仅缓慢进行。这一点通过体外翻译的苹果酸合酶被摄取到乙醛酸循环体中以及对体内乙醛酸循环体中可检测到的新合成苹果酸合酶的分析得到了证明。在这两种情况下,八聚体都是最主要的形式。

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