青贮蘑菇渣的营养品质及体外发酵特性评价

本文旨在评估蘑菇渣青贮料的营养品质、发酵特性及其与常规饲料原料的体外降解差异性。试验将收集的蘑菇渣作为原料,与米糠、糖蜜、垫料和菌种混合后青贮4周。分别在青贮0、7、14和28d时收集样品,用于评估营养品质、体外发酵特性,同时对比青贮蘑菇渣饲料与水稻秸秆和大麦秸秆的体外降解特性。结果:随着蘑菇渣青贮时间的升高,干物质含量显著降低(P<0.05),同时青贮7d后有机物含量也显著降低(P<0.05)。蘑菇渣青贮后,粗蛋白质和粗脂肪含量显著升高(P<0.05)。青贮7d后,粗灰分含量显著升高(P<0.05),而青贮7和28d后酸性洗涤纤维含量显著高于青贮0和14d(P<0.05)。蘑菇渣青贮7d后,pH显著升高(P<0.05),随后又显著降低(P<0.05),同时乙酸和丙酸含量显著降低,随后又升高(P<0.05)。蘑菇渣青贮后,乳酸和氨氮浓度显著升高(P<0.05),而水溶性碳水化物浓度显著降低(P<0.05)。青贮蘑菇渣的干物质组分中,水溶降解部分显著高于水稻秸秆和大麦秸秆(P<0.05),但不溶降解部分显著降低(P<0.05)且非降解部分显著低于水稻秸秆(P<0.05)。针对蛋白组分,青贮蘑菇渣水溶降解部分也显著高于其他两种原料(P<0.05),但不溶降解和非降解部分显著降低(P<0.05)。蘑菇渣青贮料中性洗涤纤维可消化部分显著低于水稻和大麦秸秆(P<0.05),不可消化部分则显著提高(P<0.05)。结论:以蘑菇渣为基础的青贮料发酵良好,可保存至第4周。以蘑菇渣为基础的青贮料干物质和粗蛋白质降解率远高于水稻、大麦和黑秸秆,中性洗涤纤维的降解率则相反。     

添加亚油酸条件下不同剂量硝酸钠对水牛瘤胃体外发酵脂肪酸组成及相关微生物数量的影响

为了探究添加亚油酸条件下不同剂量硝酸钠对水牛瘤胃体外发酵脂肪酸组成及相关微生物数量的影响,本试验选用3头装有永久性瘤胃瘘管的母水牛,以精粗比40∶60为底物进行瘤胃液体外发酵试验。试验组硝酸钠的浓度分别为1、2、3 mg·mL^-1,对照组不加硝酸钠,每组均添加0.25 mg·mL^-1的亚油酸,每组各5个重复。在体外培养3、6、9、12、24 h时测定产气量和甲烷产量,24 h结束培养,测定瘤胃体外发酵参数、脂肪酸含量及瘤胃微生物数量。结果表明：1）添加硝酸钠显著降低了总产气量和甲烷产量（P<0.05）;2）添加硝酸钠pH值和氨态氮（NH₃-N）含量显著升高（P<0.05）,异丁酸和异戊酸含量显著降低（P<0.05）,而对总挥发性脂肪酸（TVFA）含量无显著性影响（P>0.05）;3）添加1 mg·mL^-1硝酸钠,C18：2cis-9,trans-11、C18：2trans-10,cis-12含量和不饱和脂肪酸/饱和脂肪酸（UFA/SFA）显著高于其他组（P<0.05）,且C20：5n3 （EPA）含量显著高于添加3 mg·mL^-1硝酸钠组（P<0.05）,添加2 mg·mL^-1硝酸钠C22：6n3 （DHA）含量显著高于其他组（P<0.05）;4）添加硝酸钠组原虫数量显著低于对照组（P<0.05）,添加2、3 mg·mL^-1硝酸钠产甲烷菌数量显著低于添加1 mg·mL^-1硝酸钠组（P<0.05）,添加1 mg·mL^-1硝酸钠总细菌、真菌、溶纤维丁酸弧菌、蛋白分解丁酸弧菌、非典型丁酸弧菌、亨氏丁酸弧菌数量显著高于其他组（P<0.05）。由此可得,体外法添加1~3 mg·mL^-1硝酸钠和0.25 mg·mL^-1亚油酸在维持水牛TVFA含量不变的情况下显著降低了甲烷含量,且1 mg·mL^-1硝酸钠能促进亚油酸生成共轭亚油酸（CLA）,优化脂肪酸组成,并能增加大多数瘤胃微生物的数量。     

睾丸支持细胞的功能、分离纯化及鉴定研究进展

支持细胞对维持精子形成过程中的微环境起决定作用,它可以通过分泌功能、细胞间连接形成的血睾屏障功能以及吞噬功能等来促进精子的形成过程,其发育异常会导致不同程度的雄性生殖缺陷。基于支持细胞在雄性动物生殖过程中的作用,体外培养高纯度支持细胞可成为研究睾丸两大核心功能-精子发生和性激素分泌功能相关调节机制重要的细胞模型。此外,体外培养睾丸支持细胞也可作为生殖毒理学等新兴热点领域的细胞模型,为评估和研究环境因素对雄性生殖的影响提供便利。因此,作者系统地归纳、总结了目前关于动物支持细胞生物功能的研究及常用的体外分离纯化、培养及鉴定方法,以期为利用动物支持细胞开展雄性生殖领域的研究提供参考。     

猪圆环病毒2型灭活疫苗中病毒抗原含量实时荧光定量PCR检测方法的建立

依据GenBank公布的猪圆环病毒2型Cap基因序列,在保守区域设计特异性引物和TaqMan探针,优化反应体系,建立评价猪圆环病毒2型灭活疫苗中病毒含量的实时荧光定量PCR检测方法,对方法的特异性、敏感性和重复性进行试验,并验证灭活剂用量和灭活时间对检测结果的影响。结果显示：该方法只对猪圆环病毒2型基因有特异性扩增,其他3种对照病毒基因的扩增结果均为阴性;检测灵敏度达到10^2.0 TCID₅₀/mL,比普通PCR方法高100倍;方法的重复性好,对同一样品进行10次检测,变异系数为2.28%;不同灭活剂用量和灭活时间对结果的影响较小,不会因各厂家使用的灭活剂用量和灭活时间不同,影响疫苗对比实验的公平性。该研究成功建立了一种评价猪圆环病毒2型灭活疫苗中病毒含量的实时荧光定量PCR检测方法,用于猪圆环病毒2型灭活疫苗样品中病毒抗原含量的定量,其结果可以反映不同猪圆环病毒2型灭活疫苗样品中抗原含量差异,为研究猪圆环病毒2型灭活疫苗病毒抗原含量评估方法提供了新的思路。     

2019—2020年新疆部分地区猪PCV2的抗体水平检测及分析

为了解2019—2020年新疆地区猪圆环病毒病2型（PCV2）抗体水平及其消长规律,本试验采用间接酶联免疫吸附试验（ELISA）方法对475份血清中PCV2免疫抗体水平进行检测和分析。结果显示,PCV2抗体平均阳性率为69.68%（331/475）,未达到国家规定标准（70%）。S/P的平均值为1.56。不同类别猪群抗体平均阳性率在42.50%~86.67%之间,有一定的差异。在调查的5个规模化养殖场中,仅有2个场PCV2免疫抗体阳性率达到国家标准。各场应根据抗体检测结果,进一步对现有的免疫程序进行调整和完整,确保各猪群健康。     

Protein and energy concentrations of meat meal and meat and bone meal fed to pigs based on in vitro assays

The objective of this study was to develop equations for estimating ileal digestible crude protein (CP) and metabolizable energy (ME) contents of meat meal (MM) and meat and bone meal (MBM) as feed ingredients for pigs based on in vitro assays. Test ingredients were 4 sources of MM and 3 sources of MBM. Ash and CP contents of the ingredients ranged from 3.8% to 33.1% and 46.8% to 82.9% (as-is basis), respectively. In vitro ileal disappearance (IVID) of CP was determined and ileal digestible CP content was calculated by multiplying CP content by IVID of CP. In vitro total tract disappearance (IVTTD) of dry matter (DM) was determined and ME was calculated using gross energy, CP contents, and IVTTD of DM. The IVID of CP and IVTTD of DM ranged from 77.2% to 88.7% and from 82.7% to 92.4%, respectively. Calculated ileal digestible CP and ME contents ranged from 37.8% to 73.5% DM and 2,405 to 3,905 kcal/kg DM, respectively. Ash contents were negatively correlated (P < 0.001) with CP (r = −0.99), in vitro ileal digestible CP (r = −0.97), gross energy (r = −1.00), in vitro digestible energy (r = −0.97), and adjusted ME (r = −0.97). The most fitting equations for ileal digestible CP and adjusted ME were: ileal digestible CP (% DM) = 11.91 − 0.90 × Ash (% DM) + 0.74 × IVID of CP (%) (R² = 0.99) and adjusted ME (kcal/kg DM) = 130.85 − 50.90 × ash (% DM) + 47.06 × IVTTD of DM (%) (R² = 0.99). To validate the accuracy of the prediction equations for ME, mean bias and linear bias were determined using a regression analysis. Calculated ME values of MM and MBM were in a good agreement with data obtained from animal experiments based on a statistically insignificant bias in the models. In conclusion, ME concentrations of MM and MBM as swine feed ingredients can be calculated using ash concentration and in vitro disappearance of dry matter.     

Construction and Identification of Yeast Surface Display Libraries of Ovis aries DRA Gene Exon 2

The specific primers were designed according to Ovis aries DRA gene sequence deposited in GenBank and the multiple cloning site of the plasmid pYD1,which was a vector used for protein surface display on Saccharomyces cerevisiae.The gene encoding DRA was amplified by PCR using the genomic RNA of Ovis aries.The 762 bp fragment was cloned and released in GenBank and registration number was KR422362.The PCR product was inserted into the yeast surface display plasmid vector pYD1 by double enzyme digestion.It was indicated that DRA gene was successfully integrated into the genome.Dot mutation was made at both ends of exon 2 in DRA gene for making restriction enzyme cutting site and design the exon 2 specific primers according to mutated Ovis aries DRA gene sequence.Sequenced exon 2 amplification products based on DNA pooling of sheep large sample template was analyzed the polymorphic loci.The polymorphic exon 2 246 bp fragment was obtained by double enzyme digestion and connected to surface display restructuring mutation carriers pYD1-DRA by the same double enzyme digestion,and then we successfully constructed yeast surface display libraries.We transformed it into Saccharomyces cerevisiae EBY100 cell.Yeast monoclone was identified by PCR amplification and sequencing,and we confirmed that DRA gene had been integrated into Saccharomyces cerevisiae genome.After galactose induced,it was detected that DRA gene library had been successfully demonstrated on the yeast cell surface under the fluorescence microscope by immunofluorescence method.     

In vitro rumen fermentation and digestibility of buffaloes as influenced by grape pomace powder and urea treated rice straw supplementation

This study aimed to investigate the effect of grape pomace powder levels and roughage sources on gas kinetics, digestibility and fermentation of swamp buffaloes by using in vitro techniques. The experimental design was a 2 × 4 factorial arrangement in a completely randomized design. Factor A was two sources of roughage (untreated rice straw, RS, and 3% urea treated rice straw, UTRS) and factor B was four levels of grape pomace powder (GPP) supplementation (0, 2, 4, 6% of substrate) on a dry matter basis. Results revealed that GPP supplementation at 2, 4 and 6% of substrate influenced gas kinetics. Cumulative gas production tended to be lower in the supplemented group. In vitro true digestibility was higher in the GPP supplementation at 2% with UTRS while microbial mass was higher in the supplemented groups. Supplementation of GPP significantly increased the total volatile fatty acids, especially propionate. Calculated methane production was subsequently decreased in the supplemented groups. Bacterial population was higher while protozoal population was lower by GPP supplementation. It could be concluded that supplementation of GPP at 2% of the substrate with UTRS improved in vitro true digestibility, rumen fermentation end‐products as well as reducing methane production.