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首页> 外文期刊>Plant and cell physiology >An Activity-Staining Method on Filtration Paper Enables High-Throughput Screening of Temperature-Sensitive and Inactive Mutations of Rice alpha-Amylase for Improvement of Rice Grain Quality
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An Activity-Staining Method on Filtration Paper Enables High-Throughput Screening of Temperature-Sensitive and Inactive Mutations of Rice alpha-Amylase for Improvement of Rice Grain Quality

机译:过滤纸上的活性染色方法使得高通量筛选水稻α-淀粉酶的温度敏感和惰性突变,以提高水稻粒度

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摘要

alpha-Amylase is a starch-hydrolyzing enzyme (EC 3.2.1.1) indispensable for germination of cereal seeds, but it is also expressed during the ripening stage. Previous studies demonstrated that the enzyme is activated in developing rice seeds under extremely hot weather and triggers a loss of grain quality by hindering the accumulation of storage starch in the endosperm. Since inactive or, preferably, heatlabile alpha-amylases are preferable for breeding premium rice, we developed a method for rapid screening of inactive and temperature-sensitive mutants of the enzyme by combining the random mutagenesis by error-prone PCR and an on-filter activity test of the recombinant enzyme expressed by Escherichia coli. This technique was applied to a major alpha-amylase in the developing seed, Amy3D, and the activity of the isolated mutant enzymes was verified with both the bacteria-expressed recombinant proteins and the extract from the endosperm overexpressing each of them. Then, we identified several substitutions leading to loss of the activity of amino acid residues (Leu28, Asp112, Cys149, Trp201, Asp204, Gly295, Leu300 and Cys342), as well as a variety of heat-sensitive substitutions of Asp83, Asp187 and Glu252. Furthermore, variations of the heat-labile enzymes were created by combining these heat-sensitive mutations. The effects of the respective mutations and their relationship to the structure of the enzyme molecule are discussed.
机译:α-淀粉酶是谷物种子萌发所必需的淀粉水解酶(EC 3.2.1.1),但在成熟阶段也有表达。先前的研究表明,在极端炎热的天气下,这种酶在水稻种子发育过程中被激活,并通过阻碍胚乳中贮藏淀粉的积累而引发稻米品质的损失。由于非活性或不耐热α-淀粉酶是选育优质水稻的首选酶,我们开发了一种方法,通过结合易出错PCR的随机突变和大肠杆菌表达的重组酶的过滤活性试验,快速筛选非活性和温度敏感的酶突变体。该技术被应用于发育中种子中的一种主要α-淀粉酶Amy3D,分离出的突变酶的活性通过细菌表达的重组蛋白和胚乳中过度表达每一种蛋白的提取物进行了验证。然后,我们确定了导致氨基酸残基活性丧失的几种替代物(Leu28、Asp112、Cys149、Trp201、Asp204、Gly295、Leu300和Cys342),以及Asp83、Asp187和Glu252的多种热敏替代物。此外,通过结合这些热敏突变,产生了耐热酶的变异。讨论了各自突变的影响及其与酶分子结构的关系。

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