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Probing the Crucial Role of Leu31 and Thr33 of the Bacillus pumilus CBS Alkaline Protease in Substrate Recognition and Enzymatic Depilation of Animal Hide

机译:探索短小芽孢杆菌CBS碱性蛋白酶的Leu31和Thr33在底物识别和动物皮酶脱毛中的关键作用

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摘要

The sapB gene, encoding Bacillus pumilus CBS protease, and seven mutated genes (sapB-L31I, sapB-T33S, sapB-N99Y, sapB-L31I/T33S, sapB-L31I/N99Y, sapB-T33S/N99Y, and sapB-L31I/T33S/N99Y) were overexpressed in protease-deficient Bacillus subtilis DB430 and purified to homogeneity. SAPB-N99Y and rSAPB displayed the highest levels of keratinolytic activity, hydrolysis efficiency, and enzymatic depilation. Interestingly, and at the semi-industrial scale, rSAPB efficiently removed the hair of goat hides within a short time interval of 8 h, thus offering a promising opportunity for the attainment of a lime and sulphide-free depilation process. The efficacy of the process was supported by submitting depilated pelts and dyed crusts to scanning electron microscopic analysis, and the results showed well opened fibre bundles and no apparent damage to the collagen layer. The findings also revealed better physico-chemical properties and less effluent loads, which further confirmed the potential candidacy of the rSAPB enzyme for application in the leather industry to attain an ecofriendly process of animal hide depilation. More interestingly, the findings on the substrate specificity and kinetic properties of the enzyme using the synthetic peptide para-nitroanilide revealed strong preferences for an aliphatic amino-acid (valine) at position P1 for keratinases and an aromatic amino-acid (phenylalanine) at positions P1/P4 for subtilisins. Molecular modeling suggested the potential involvement of a Leu31 residue in a network of hydrophobic interactions, which could have shaped the S4 substrate binding site. The latter could be enlarged by mutating L31I, fitting more easily in position P4 than a phenylalanine residue. The molecular modeling of SAPB-T33S showed a potential S2 subside widening by a T33S mutation, thus suggesting its importance in substrate specificity.
机译:编码短小芽孢杆菌CBS蛋白酶的sapB基因和七个突变基因(sapB-L31I,sapB-T33S,sapB-N99Y,sapB-L31I / T33S,sapB-L31I / N99Y,sapB-T33S / N99Y和sapB- T33S / N99Y)在蛋白酶缺陷型枯草芽孢杆菌DB430中过表达并纯化至均一。 SAPB-N99Y和rSAPB显示出最高水平的角蛋白分解活性,水解效率和酶促脱毛作用。有趣的是,在半工业规模上,rSAPB在8小时的短时间内有效地去除了山羊皮的毛发,从而为实现无石灰和无硫化物的脱毛工艺提供了一个有希望的机会。通过对脱毛的毛皮和染色的皮进行扫描电子显微镜分析来支持该方法的有效性,结果表明,纤维束充分开放,对胶原层没有明显损害。这些发现还揭示了更好的理化特性和更少的废水负荷,这进一步证实了rSAPB酶在皮革工业中的潜在候选资格,以实现生态友好的动物皮脱毛工艺。更有趣的是,使用合成肽对硝基苯胺对酶的底物特异性和动力学性质的发现表明,对于角蛋白酶而言,P1位的脂族氨基酸(缬氨酸)和角蛋白位置的芳族氨基酸(苯丙氨酸)具有强烈的偏好性。枯草杆菌蛋白酶的P1 / P4。分子建模表明,Leu31残基可能参与了疏水相互作用的网络,该相互作用可能已经塑造了S4底物的结合位点。后者可以通过突变L31I来扩大,比苯丙氨酸残基更容易插入P4位。 SAPB-T33S的分子模型显示,由于T33S突变,潜在的S2消退变宽,因此表明其在底物特异性中的重要性。

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