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Identification of amino acid residues critical for catalysis and stability in Aspergillus niger family 1 pectin lyase A.

机译：在黑曲霉家族1果胶裂解酶A中对催化和稳定性至关重要的氨基酸残基的鉴定。

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摘要

Site-directed-mutagenesis studies were performed on family 1 pectin lyase A (PL1A) from Aspergillus niger to gain insight into the reaction mechanism for the pectin lyase-catalysed beta-elimination cleavage of methylesterified polygalacturonic acid and to stabilize the enzyme at slightly basic pH. On the basis of the three-dimensional structures of PL1A [Mayans, Scott, Connerton, Gravesen, Benen, Visser, Pickersgill and Jenkins (1997) Structure 5, 677-689] and the modelled enzyme-substrate complex of PL1B [Herron, Benen, Scavetta, Visser and Jurnak (2000) Proc. Natl. Acad. Sci. U.S.A. 97, 8762-8769], Asp154, Arg176, Arg236 and Lys239 were mutagenized. Substituting Arg236 with alanine or lysine rendered the enzyme completely inactive, and mutagenesis of Arg176 and Lys239 severely affected catalysis. The Asp154-->Arg and Asp154-->Glu mutant enzymes were only moderately impaired in respect of catalysis. The results strongly indicate that Arg236, which is sandwiched between Arg176 and Lys239, would initiate the reaction upon enzyme-substrate interaction, through the abstraction of the proton at C5 of the galacturonopyranose ring. The positively charged residues Arg176 and Lys239 are responsible for lowering the p K a of Arg236. Arg176 and Lys239 are maintained in a charged state by interacting with Asp154 or bulk solvent respectively. The deprotonation of the Asp186-Asp221 pair was proposed to be responsible for a pH-driven conformational change of PL1A [Mayans, Scott, Connerton, Gravesen, Benen, Visser, Pickersgill and Jenkins (1997) Structure 5, 677-689]. Substitution of Asp186 and Asp221 by Asn186 and Asn221 was expected to stabilize the enzyme. However, the Asp186-->Asn/Asp221-->Asn enzyme appeared less stable than the wild-type enzyme, even at pH 6.0, as evidenced by fluorescence studies. This demonstrates that the pH-dependent conformational change is not driven by deprotonation of the Asp186-Asp221 pair.

机译：对来自黑曲霉的1号家庭果胶裂解酶A（PL1A）进行了定点诱变研究，以深入了解果胶裂解酶催化β-消除甲基酯化的聚半乳糖醛酸的反应机理，并将该酶稳定在基本碱性的pH下。基于PL1A的三维结构[Mayans，Scott，Connerton，Gravesen，Been，Visser，Pickersgill和Jenkins（1997）Structure 5，677-689]和PL1B的酶-底物复合物模型[Herron，Benen ，Scavetta，Visser和Jurnak（2000）Proc。 Natl。学院科学[U.S.A. 97，8762-8769]，Asp154，Arg176，Arg236和Lys239进行了诱变。用丙氨酸或赖氨酸取代Arg236使该酶完全失活，并且诱变Arg176和Lys239严重影响了催化作用。在催化方面，Asp154-> Arg和Asp154-> Glu突变酶仅受到中等程度的损害。结果强烈表明，夹在Arg176和Lys239之间的Arg236将通过提取半乳糖醛酸吡喃糖环C5处的质子来引发酶-底物相互作用后的反应。带正电的残基Arg176和Lys239负责降低Arg236的p K a。 Arg176和Lys239分别通过与Asp154或本体溶剂相互作用而保持带电状态。有人提出Asp186-Asp221对的去质子化是造成pH驱动的PL1A构象变化的原因[Mayans，Scott，Connerton，Gravesen，Benen，Visser，Pickersgill and Jenkins（1997）Structure 5，677-689]。预期Asn186和Asn221取代Asp186和Asp221可稳定该酶。但是，Asp186-> Asn / Asp221-> Asn酶的稳定性比野生型酶差，甚至在pH 6.0时也是如此。这证明pH依赖性构象变化不是由Asp186-Asp221对的去质子化驱动的。

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Sánchez-Torres, Paloma; Visser, Jaap; Benen, Jacques A E;
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年度 2003
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1. Identification of amino acid residues critical for catalysis and stability in Aspergillus niger family 1 pectin lyase A. [J] . Sanchez Torres P, Visser J, Benen JA The Biochemical Journal . 2003,第Pta1期

机译：在黑曲霉家族1果胶裂解酶A中对催化和稳定性至关重要的氨基酸残基的鉴定。
2. Identification of amino acid residues critical for catalysis and stability in Aspergillus niger family 1 pectin lyase A [J] . Jaap VISSER, Jacques A.E. BENEN, Paloma SáNCHEZ-TORRES The biochemical journal . 2003,第1期

机译：黑曲霉家族1果胶裂解酶A的催化和稳定性至关重要的氨基酸残基的鉴定
3. Identification of amino acid residues critical for catalysis and stability in Aspergillus niger family 1 pectin lyase A [J] . Sanchez-Torres P, Visser J, Benen JAE The Biochemical Journal . 2003,第0期

机译：黑曲霉家族1果胶裂解酶A的催化和稳定性至关重要的氨基酸残基的鉴定
4. Aspergillus flavus, A. niger, A. ochraceus AND A. parasiticus INHIBITION BY MICROWAVE HEATING AT SELECTED WATER ACTIVITIES [C] . Cruz-Guerrero G., Sosa-Morales M. E., Lopez-Malo A. International Microwave Power Institute's Annual Symposium . 2008

机译：曲霉菌，A.尼日尔，A. Ochraceus和A.通过微波加热在所选水上活动的寄生菌抑制
5. Identification of Amino Acid Residues Critical for TLR3 Inhibition by the Multifunctional West Nile Virus NS1 Protein. [D] . Morrison, Clayton Russell. 2013

机译：鉴定多功能西尼罗河病毒NS1蛋白对TLR3抑制至关重要的氨基酸残基。
6. Identification of amino acid residues critical for catalysis and stability in Aspergillus niger family 1 pectin lyase A. [O] . Paloma Sánchez-Torres, Jaap Visser, Jacques A E Benen 2003

机译：在黑曲霉家族1果胶裂解酶A中对催化和稳定性至关重要的氨基酸残基的鉴定。
7. Identification of amino acid residues responsible for increased thermostability of feruloyl esterase A from Aspergillus niger using the PoPMuSiC algorithm [O] . Zhang Shuai-Bing, Wu Zhong-Liu 2011

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