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玉米籽粒盾片中脂肪酶的生物合成。

Biosynthesis of lipase in the scutellum of maize kernel.

作者信息

Wang S M, Huang A H

出版信息

J Biol Chem. 1987 Feb 15;262(5):2270-4.

PMID:2434479
Abstract

In the scutellum of maize kernel after imbibition, lipase activity increased rapidly, concomitant with the decrease in storage triacylglycerols. The enzyme activity peaked at day 6, but remained at the same level from day 6-10 when most of the triacylglycerols had been depleted. By in vitro translation with extracted RNAs followed by immunoprecipitation, and by resolving the translation products by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, lipase was found to be de novo synthesized in postgermination. The enzyme was synthesized by RNAs extracted from free polyribosomes and not from bound polyribosomes. Both in vitro and in vivo synthesized lipase had the same Mr of 65,000 as resolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, as had the purified authentic enzyme; thus there was no appreciable co- or post-translational processing of the enzyme. Lipase-specific mRNA was present only between day 2-6 after imbibition. At day 6 when lipolysis was most active, more than 60% of the lipase activity was recovered in the lipid body fraction and specifically associated with the organelle membrane. From day 6-10, the lipase activity gradually shifted from the lipid body fraction to other subcellular fractions, including the 10,000 X g pellet, the 120,000 X g pellet, and the 120,000 X g supernatant. Lipase in these subcellular fractions was attributed to represent the enzyme associated with membrane ghosts of the lipid bodies which were fusing with the fragile cell vacuoles; such fusions were observed in situ by electron microscopy.

摘要

在玉米籽粒吸胀后的盾片中,脂肪酶活性迅速增加,同时储存的三酰甘油减少。该酶活性在第6天达到峰值,但在第6 - 10天,当大部分三酰甘油已被耗尽时,活性保持在相同水平。通过用提取的RNA进行体外翻译,随后进行免疫沉淀,并通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳分离翻译产物,发现脂肪酶是在种子萌发后从头合成的。该酶是由从游离多核糖体而非结合多核糖体提取的RNA合成的。体外和体内合成的脂肪酶,经十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳解析,其分子量均为65,000,与纯化的天然酶相同;因此该酶没有明显的共翻译或翻译后加工。脂肪酶特异性mRNA仅在吸胀后第2 - 6天存在。在脂肪分解最活跃的第6天,超过60%的脂肪酶活性在脂质体组分中回收,并特异性地与细胞器膜相关联。从第6 - 10天,脂肪酶活性逐渐从脂质体组分转移到其他亚细胞组分,包括10,000×g沉淀、120,000×g沉淀和120,000×g上清液。这些亚细胞组分中的脂肪酶被认为代表了与正在与脆弱的细胞液泡融合的脂质体膜空壳相关的酶;通过电子显微镜在原位观察到了这种融合。

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