首页> 外文期刊>Canadian Journal of Animal Science >Effect of dried distillers' grains and solubles when replacing corn or soybean meal on rumen microbial growth in vitro as measured using DNA as a microbial marker.
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Effect of dried distillers' grains and solubles when replacing corn or soybean meal on rumen microbial growth in vitro as measured using DNA as a microbial marker.

机译:用DNA作为微生物标记物测得的干酒糟和可溶物在替代玉米或豆粕时对瘤胃微生物体外生长的影响。

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The objectives were to evaluate the use of rDNA markers to measure the effects of dried distillers' grains with solubles (DDGS) and the potential treatment x time interaction on microbial crude protein (MCP) synthesis in vitro and secondly to measure the contribution of yeast based protein originating from DDGS. Treatments were: (1) CONT, control with no DDGS, but with alfalfa hay, corn silage, ground corn (GC) and soybean meal (SBM) included at 25% (DM basis); (2) LOWCORN, 20% DDGS (DM basis) replacing GC; (3) LOWSBM, 20% DDGS (DM basis) replacing SBM; and (4) LOWCORNSBM, 20% DDGS (DM basis) replacing 10% GC and 10% SBM. Treatments (0.5 g) were incubated in 50 mL of inoculum in duplicate. At 0, 4, 16, 32, 48 and 96 h of fermentation total DNA was extracted from each treatment and MCP was measured using rDNA markers. The sum of bacterial crude protein (BCP) and protozoal crude protein (PCP) was considered as MCP. Data were analyzed as a completely randomized design. The treatment x time interaction was tested and the SLICE option was included to evaluate the effect of treatment at each fermentation time point. There was a tendency to a treatment x time interaction (P=0.07) for MCP. Specifically, at 16 h, LOWCORNSBM yielded greater (P<0.05) MCP compared to either CONT or LOWCORN with estimates of 68.5, 33.8 and 23.3+or-8.9 mg g-1 DM, for LOWCORNSBM, CONT and LOWCORN, respectively. At 48 h, however, LOWCORN yielded greater MCP (P<0.05) compared with LOWSBM with estimates of 72.2 and 32.5+or-8.9 mg g-1 DM, for LOWCORN and LOWSBM, respectively. Yeast crude protein (YCP) was not affected (P=0.21) and averaged 0.04+or-0.02 mg g-1 of substrate (DM basis). Overall, rDNA markers were effective for quantifying MCP, but further research on the methodology is needed. With DDGS inclusion, MCP was maintained; however, yeast cells were extensively degraded during fermentation.
机译:目的是评估使用rDNA标记物测量干酒糟含可溶性物质(DDGS)的效果以及潜在的x时间相互作用对体外微生物粗蛋白(MCP)合成的影响,其次用于测量基于酵母的酵母的贡献来自DDGS的蛋白质。处理方法为:(1)CONT,无DDGS的对照,但以25%(以DM为基准)包括苜蓿干草,玉米青贮饲料,玉米粉(GC)和豆粕(SBM); (2)LOWCORN,20%DDGS(基于DM)代替GC; (3)LOWSBM,用20%DDGS(以DM为基础)代替SBM; (4)LOWCORNSBM,20%DDGS(以DM为基础)代替10%GC和10%SBM。将处理物(0.5 g)一式两份在50 mL接种物中孵育。在发酵的0、4、16、32、48和96 h时,从每种处理中提取总DNA,并使用rDNA标记物测量MCP。细菌粗蛋白(BCP)和原生动物粗蛋白(PCP)的总和被认为是MCP。数据作为完全随机设计进行分析。测试了处理与时间的交互作用,并包括了SLICE选项以评估每个发酵时间点的处理效果。 MCP有治疗x时间相互作用(P = 0.07)的趋势。具体而言,与CONT或LOWCORN相比,LOWCORNSBM在16 h产生的MCP更大(P <0.05),估计LOWCORNSBM,CONT分别为68.5、33.8和23.3+或-8.9 mg g -1 DM和LOWCORN。然而,与LOWSBM相比,LOWCORN在48 h产生的MCP更大(P <0.05),估计LOWCORN和LOWSBM分别为72.2和32.5+或-8.9 mg g -1 DM。酵母粗蛋白(YCP)未受影响(P = 0.21),平均底物平均为0.04+或-0.02 mg g -1 (以DM为基准)。总体而言,rDNA标记对于定量MCP有效,但仍需要对该方法进行进一步研究。包含DDGS后,MCP得以保留;然而,酵母细胞在发酵过程中被广泛降解。

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