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豌豆种子中的核糖核酸合成和活力丧失。

Ribonucleic acid synthesis and loss of viability in pea seed.

机构信息

Department of Biochemistry, University of Manchester, M13 9PL, Manchester, U.K..

出版信息

Planta. 1976 Jan;132(2):103-8. doi: 10.1007/BF00388890.

Abstract

RNA synthesis and protein synthesis in embryonic axis tissue of viable pea (Pisum arvense L. var. N.Z. maple) seed commences during the first hour of germination. Protein synthesis in axis tissue of non-viable pea seed is barely detectable during the first 24 h after the start of imbibition. Nonviable axis tissue incorporates significant levels of [(3)H]uridine into RNA during this period but the level of incorporation does not increase significantly over the first 24 h of imbibition. In axis tissue of non-viable seed during the first hour of imbibition most of the [(3)H]uridine was incorporated into low molecular weight material migrating in advance of the 4S and 5S RNA species in polyacrylamide gels but some radioactivity was incorporated into a discrete species of RNA having a molecular weight of 2.7×10(6). After 24 h, non-viable axis tissue incorporates [(3)H]uridine into ribosomal RNA, the low molecular weight material migrating in advance of the 4S and 5S RNA peak in polyacrylamide gels and a heterogeneous RNA species of molecular weight ranging from 2.2×10(6) to 2.7×10(6). No 4S or 5S RNA synthesis is detectable after 24 h of imbibition in non-viable axis tissue. Axis tissue of viable pea seed synthesises rRNA, 4S and 5S RNA, the low molecular weight material migrating in advance of the 4S and 5S RNA peak in polyacrylamide gels and the rRNA precursor species at both periods of germination studied. Loss of viability in pea seed appears to be accompanied by the appearance of lesions in the processing of rRNA precursor species and a significant loss of RNA synthesising activity.

摘要

活体豌豆(Pisum arvense L. var. N.Z. maple)种子胚轴组织中的 RNA 合成和蛋白质合成在萌发的第一个小时内开始。在吸胀开始后的前 24 小时内,非活体豌豆种子的胚轴组织中几乎检测不到蛋白质合成。在此期间,非活体胚轴组织将大量 [(3)H]尿嘧啶掺入 RNA 中,但在吸胀的前 24 小时内,掺入量没有显著增加。在吸胀的第一个小时内,非活体种子的胚轴组织中,大多数 [(3)H]尿嘧啶被掺入到聚丙烯酰胺凝胶中比 4S 和 5S RNA 先迁移的低分子量物质中,但一些放射性被掺入到分子量为 2.7×10(6)的离散 RNA 物种中。24 小时后,非活体胚轴组织将 [(3)H]尿嘧啶掺入核糖体 RNA、聚丙烯酰胺凝胶中比 4S 和 5S RNA 峰先迁移的低分子量物质以及分子量范围从 2.2×10(6)到 2.7×10(6)的异质 RNA 物种中。在非活体胚轴组织中,吸胀 24 小时后,无法检测到 4S 或 5S RNA 的合成。活体豌豆种子的胚轴组织合成 rRNA、4S 和 5S RNA、聚丙烯酰胺凝胶中比 4S 和 5S RNA 峰先迁移的低分子量物质以及在两个萌发期研究的 rRNA 前体物种。豌豆种子的活力丧失似乎伴随着 rRNA 前体物种加工过程中出现损伤和 RNA 合成活性的显著丧失。

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