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Application of standard addition for the determination of carboxypeptidase activity in Actinomucor elegans bran koji

机译:标准添加物在放线放线杆菌麸曲中羧肽酶活性测定中的应用

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Leucine carboxypeptidase (EC 3.4.16) activity in Actinomucor elegans bran koji was investigated via absorbance at 507 nm after stained by Cd-nihydrin solution, with calibration curve A, which was made by a set of known concentration standard leucine, calibration B, which was made by three sets of known concentration standard leucine solutions with the addition of three concentrations inactive crude enzyme extract, and calibration C, which was made by three sets of known concentration standard leucine solutions with the addition of three concentrations crude enzyme extract. The results indicated that application of pure amino acid standard curve was not a suitable way to determine carboxypeptidase in complicated mixture, and it probably led to overestimated carboxypeptidase activity. It was found that addition of crude exact into pure amino acid standard curve had a significant difference from pure amino acid standard curve method (p < 0.05). There was no significant enzyme activity difference (p > 0.05) between addition of active crude exact and addition of inactive crude kind, when the proper dilute multiple was used. It was concluded that the addi-tion of crude enzyme extract to the calibration was needed to eliminate the interference of free amino acids and related compounds presented in crude enzyme extract.
机译:通过镉-三羟甲基氨基甲烷溶液染色后,通过在507 nm处的吸光度研究Actinomucor elegans bran koji中的亮氨酸羧肽酶(EC 3.4.16)活性,其校准曲线A由一组已知浓度的标准亮氨酸(校准B)制成。用三组已知浓度的标准亮氨酸溶液加三浓度的非活性粗酶提取物制得标样C,并用三组已知浓度的标准亮氨酸溶液加三浓度的粗酶提取物制得标样C。结果表明,应用纯氨基酸标准曲线并不是测定复杂混合物中羧肽酶的合适方法,可能会导致高估羧肽酶的活性。结果发现,在纯氨基酸标准曲线中添加精确的粗品与纯氨基酸标准曲线方法有显着差异(p <0.05)。当使用适当的稀释倍数时,精确添加活性原油和添加非活性原油之间没有显着的酶活性差异(p> 0.05)。结论是需要将粗酶提取物添加到标定中,以消除粗酶提取物中存在的游离氨基酸和相关化合物的干扰。

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