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New recombinant fibrolytic enzymes for improved in vitro ruminal fiber degradability of barley straw

机译:改善大麦秸秆体外瘤胃纤维降解性的新型重组纤溶酶

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摘要

This study used a high-throughput in vitro microassay, in vitro batch culture, and the Rumen Simulation Technique (>RUSITEC) to screen recombinant fibrolytic enzymes for their ability to increase the ruminal fiber degradability of barley straw. Eleven different recombinant enzymes in combination with a crude mixture of rumen enzymes (50% recombinant enzyme:50% crude mixture of rumen enzymes) were compared with the crude mixture of rumen enzymes alone. In the microassay, all treatments were applied at 15 mg of protein load per gram barley straw glucan. Based on the microassay results, 1 recombinant endoglucanase [EGL7A, from the glycoside hydrolase (>GH) family 7], 2 recombinant xylanases (XYL10A and XYL10C, from GH10), and a recombinant enzyme mixture were selected and compared with a crude mixture of fibrolytic enzymes from Aspergillus aculeatus for their ability to hydrolyze barley straw. For batch culture, enzymes were applied to barley straw at 2 dosages (100 and 500 µg of protein/g of substrate DM). All enzymes increased (P < 0.05) DM disappearance and total VFA production, but the mixture of recombinant enzymes was not superior to the use of a single recombinant enzyme. Based on positive results (P < 0.05) for total DM disappearance and VFA production in batch culture, 3 enzymes (EGL7A, XYL10A, and XYL10C) were selected and applied to barley straw at 500 µg of protein per gram for further assessment in RUSITECs fed a concentrate:barley straw diet (300:700 g/kg DM). In RUSITECs, the recombinant enzyme XYL10A increased (P < 0.05) barley straw DM, NDF, and ADF disappearance, whereas EGL7A and XYL10C had no effect. The enzymes selected based on the high-throughput in vitro microassay consistently increased barley straw degradation in ruminal batch culture, but not in the semicontinuous culture RUSITEC system.
机译:这项研究使用高通量的体外显微测定,体外分批培养和Rumen模拟技术(> RUSITEC )来筛选重组纤维分解酶提高大麦秸秆瘤胃纤维降解能力的能力。将十一种不同的重组酶与瘤胃酶的粗混合物(50%重组酶:50%瘤胃酶的粗混合物)组合,与单独的瘤胃酶的粗混合物进行比较。在微量测定中,所有处理均以每克大麦秸秆葡聚糖15毫克蛋白质负载的量进行。根据微观分析结果,选择了1种重组糖苷内切酶[EGL7A,来自糖苷水解酶(> GH )家族7],2种重组木聚糖酶(XYL10A和XYL10C,来​​自GH10)和重组酶混合物,与来自棘​​孢曲霉的纤维分解酶的粗混合物相比,它们具有水解大麦秸秆的能力。对于分批培养,将酶以2种剂量(100和500 µg蛋白质/ g底物DM)施加到大麦秸秆上。所有酶均增加(P <0.05)DM消失和总VFA产生,但重组酶的混合物并不优于单一重组酶的使用。根据分批培养中总DM消失和VFA产生的阳性结果(P <0.05),选择了3种酶(EGL7A,XYL10A和XYL10C),并以每克500 µg蛋白质的浓度将其应用于大麦秸秆,以便在RUSITEC中进行进一步评估浓缩物:大麦秸秆饮食(300:700 g / kg DM)。在RUSITEC中,重组酶XYL10A增加了(P <0.05)大麦秸秆DM,NDF和ADF的消失,而EGL7A和XYL10C没有作用。基于高通量体外显微分析的酶在瘤胃分批培养中始终提高大麦秸秆的降解,但在半连续培养RUSITEC系统中则没有。

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