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New Insights into the Fructosyltransferase Activity of Schwanniomyces occidentalis β-Fructofuranosidase, Emerging from Nonconventional Codon Usage and Directed Mutation

机译:非常规密码子使用和定向突变产生的新发现的西方西门氏菌β-果糖呋喃糖苷酶果糖基转移酶活性的新见解

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Schwanniomyces occidentalis β-fructofuranosidase (Ffase) releases β-fructose from the nonreducing ends of β-fructans and synthesizes 6-kestose and 1-kestose, both considered prebiotic fructooligosaccharides. Analyzing the amino acid sequence of this protein revealed that it includes a serine instead of a leucine at position 196, caused by a nonuniversal decoding of the unique mRNA leucine codon CUG. Substitution of leucine for Ser196 dramatically lowers the apparent catalytic efficiency ( k _(cat)/ K_(m) ) of the enzyme (approximately 1,000-fold), but surprisingly, its transferase activity is enhanced by almost 3-fold, as is the enzymes' specificity for 6-kestose synthesis. The influence of 6 Ffase residues on enzyme activity was analyzed on both the Leu196/Ser196 backgrounds (Trp47, Asn49, Asn52, Ser111, Lys181, and Pro232). Only N52S and P232V mutations improved the transferase activity of the wild-type enzyme (about 1.6-fold). Modeling the transfructosylation products into the active site, in combination with an analysis of the kinetics and transfructosylation reactions, defined a new region responsible for the transferase specificity of the enzyme.
机译:西方Schwanniomyces occidentalisβ-果糖呋喃糖苷酶(Ffase)从β-果糖的非还原末端释放β-果糖,并合成6-果糖和1-Kest​​ose,两者均被认为是益生元低聚果糖。分析该蛋白的氨基酸序列,发现其在位置196处包含丝氨酸而不是亮氨酸,这是由独特的mRNA亮氨酸密码子CUG的非普遍解码引起的。亮氨酸替换为Ser196会大大降低该酶的表观催化效率(k_(cat)/ K_(m))(约1,000倍),但令人惊讶的是,它的转移酶活性提高了近3倍,因为酶对6-核糖合成的特异性。在两个Leu196 / Ser196背景(Trp47,Asn49,Asn52,Ser111,Lys181和Pro232)上分析了6个Ffase残基对酶活性的影响。仅N52S和P232V突变可提高野生型酶的转移酶活性(约1.6倍)。将反果糖基化产物模拟到活性位点,结合动力学和反果糖基化反应的分析,定义了负责该酶转移酶特异性的新区域。

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