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盐对大麦根中蛋白质合成模式的影响。

The effects of salt on the pattern of protein synthesis in barley roots.

作者信息

Hurkman W J, Tanaka C K

机构信息

United States Department of Agriculture, Western Regional Research Center, Albany, California 94710.

出版信息

Plant Physiol. 1987 Mar;83(3):517-24. doi: 10.1104/pp.83.3.517.

Abstract

The effect of salt stress on the incorporation of [(35)S]methionine into protein was examined in roots of barley (Hordeum vulgare L. cv California Mariout 72). Plants were grown in nutrient solution with or without 200 millimolar NaCl. Roots of intact plants were labeled in vivo and proteins were extracted and analyzed by fluorography of two-dimensional gels. Although the protein patterns for control and salt-stressed plants were qualitatively similar, the net synthesis of a number of proteins was quantitatively changed. The most striking change was a significant increase of label in two protein pairs that had pIs of approximately 6.3 and 6.5. Each pair consisted of proteins of approximately 26 and 27 kilodaltons (kD). In roots of control plants, the 27-kD proteins were more heavily labeled in the microsomal fraction relative to the 26-kD proteins, whereas the 26-kD proteins were enriched in the post 178,000 g supernatant fraction; in roots of salt treated plants, the 26- and 27-kD proteins were more intensely labeled in both fractions. Labeling of the 26- and 27-kD proteins returned to control levels when salt-stressed plants were transferred to nutrient solution without NaCl. No cross-reaction was detected between the antibody to the 26-kD protein from salt-adapted tobacco cells and the 26- and 27-kD proteins of barley.

摘要

在大麦(Hordeum vulgare L. cv California Mariout 72)的根中研究了盐胁迫对[(35)S]甲硫氨酸掺入蛋白质的影响。将植物种植在含有或不含有200毫摩尔氯化钠的营养液中。完整植株的根在体内进行标记,然后提取蛋白质,并通过二维凝胶荧光自显影进行分析。尽管对照植株和盐胁迫植株的蛋白质图谱在定性上相似,但一些蛋白质的净合成在数量上发生了变化。最显著的变化是两组蛋白质(其等电点约为6.3和6.5)的标记显著增加。每组由分子量约为26和27千道尔顿(kD)的蛋白质组成。在对照植株的根中,相对于26-kD蛋白质,27-kD蛋白质在微粒体部分的标记更重,而26-kD蛋白质在178,000 g上清液部分中富集;在盐处理植株的根中,26-kD和27-kD蛋白质在这两个部分中的标记都更强。当盐胁迫植株转移到不含氯化钠的营养液中时,26-kD和27-kD蛋白质的标记恢复到对照水平。在来自盐适应烟草细胞的26-kD蛋白质抗体与大麦的26-kD和27-kD蛋白质之间未检测到交叉反应。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b350/1056397/75d4e3e2cf4b/plntphys00611-0073-a.jpg

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