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日粮类型和羊草细度对肉牛瘤胃挥发性脂肪酸比例及能量转化效率的影响 总被引:6,自引:0,他引:6
用装有瘤胃瘘管和真胃瘘管的肥育阉牛,按完全拉丁方设计,连续定点消化道食糜采样,用KB-1型自控大型呼吸测热室测定能量平衡和氮平衡。结果表明,4种不同加工细度羊草,在维持饲养水平(1M)下的DE/GE,ME/DE,HP/ME,Km,VFA总量,乙酸:丙酸比例等的组间差异均不显著(P>0.05),代谢能转化为维持净能效率(Km)平均为65.69%(C.V=0.88%);1.3M饲养水平的各种能量参数,4组间的差异亦均不显著(P>0.05),代谢能转化为增重净能效率(Kf)平均33.92%(C.V=1.86%)。4种不同精料:羊草比例的日粮,在维持饲养水平下,CH4(KJ)/DE(KJ)=0.0738+0.0615(NDF/OM),r=0.8928,Km=60.8651+0.3304(丙酸mol/100molVFA),r=0.9955;在1.5M下,HP/ME=14.3838+0.7805(乙酸mol/100molVFA),r=0.9903,Kf=22.9697+0.6022(丙酸mol/100molVFA),r=0.9981,或Kf=57.2265-0.3817(NDF/OM),r=-0.9987。 相似文献
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本文选用10株NDV疫苗、10株NDV/IBV联苗,察接种2周龄雏鸡后对头部相关淋巴组织(HALT)的影响。通过对接种鸡进行一系列体内试验,检测了哈德氏腺(GH)对布氏杆菌灭活抗原滴眼的反应情况。根据这一结果,对HALT的几个部位和支气管进行组织学检查,并见到有微观变化。本研究表明:3种NDV/IBV联苗(1株B1/Mass&Conn、2株LaSota/Mass&Conn)可干扰GH对布氏抗原的反 相似文献
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筛选家蚕分子标记的有效方法—SADF法 总被引:1,自引:0,他引:1
从家蚕品种 C108 和大造后部丝腺提取的基因组 D N A 用 Pst Ⅰ酶解后与自行设计的人工接头相连,并用与人工接头序列相匹配的选择性引物进行选择性 P C R 扩增( Selective Am plification) 。扩增产物经琼脂糖凝胶电泳检测显示,用 S A D F 法在两品种中能检测到稳定的 D N A 多态性片段,表明此方法可用于分子标记的筛选。经研究发现:当 P C R 反应体系中 Mg2 + 为15 m m ol/ L,d N T Ps 为200μm ol/ L,引物为1μm ol/ L 时可得到较好的结果;在热循环过程中,以56 ℃退火为宜;扩增反应对模板 D N A 质的要求远胜于量。 相似文献
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本试验用抗 P R R S V 单克隆抗体( S D O W 17)建立了检测猪体内 P R R S V 抗原的免疫组化染色法,主要步骤:组织块在100 m L/ L中性缓冲液福尔马林中固定24~48 h→常规脱水、石蜡包埋、切片4~5μm →二甲苯脱蜡→100% 酒精→10 m L/ L盐酸酒精 30 m in(消除内源性过氧化物酶)→95% 酒精→85% 酒精→75% 酒精→蒸馏水→0.01 m ol/ L P B S→10% 马血清37 ℃30 m in 后转4 ℃过夜→0.01 m ol/ L P B S3×5 m in→生物素化马抗鼠 Ig G(1∶200) 37 ℃ 60 m in→0.01 m ol/ L P B S3× 5 m in→辣根酶标记链亲和素(1∶200)37℃ 60 m in→0.01 m ol/ L P B S3×5 m in→新鲜配制的 D A B室温下显色 5~15 m in→0.01 m ol/ L P B S洗→常规脱水、透明、封片。经对8 例试验感染 P R R S V 仔猪各种组织内 P R R S V 抗原的检测,本法具有简单、快速、特异性强,结果清晰、稳定及重复性好等特点,是检测组织内 P R R S V 抗原的一种好方法。 相似文献
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本试验对1日龄感染鸡传染性贫血病毒(CIAV)雏鸡接种新城疫(ND)疫苗及其强毒攻击后外周血液免疫球蛋白IgG、IgM、IgA含量和HI抗体滴度的动态变化进行研究。结果发现,CIAV感染雏鸡ND疫苗免疫后,其外周血液IgG、IgM、IgA含量和HI抗体滴度,于接种ND疫苗后7 ̄28d较未感染CIAV的免疫对照雏鸡明显减少,表明CIAV感染雏鸡对ND疫苗免疫的体液免疫应答功能明显降低。ND强毒攻击后 相似文献
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猪细小病毒生物学特性研究 总被引:2,自引:0,他引:2
应用PK-15传代细胞复制猪细小病毒(PPV)参考株NADL-2和云南分离株KM,研究得出细胞培养物半数细胞感染量分别为10^-7.9/ml和10^-6.8/ml经CsCl密度梯度离心,两种病毒颗粒其浮力密度值分别为1.33g/cm^3和1.39/cm,电镜观察病毒粒子呈圆形,直径约20nm。SDS-聚丙烯酰胺凝胶电泳(SDS-PAGE)分析,表明纯化的PPV细胞培养毒,主要含两种蛋白成分,分子量 相似文献
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犬瘟热病毒抗体检测方法的比较研究 总被引:19,自引:0,他引:19
用犬瘟热(CD)弱毒和自制的高免犬血清,建立了检测犬瘟热病毒(CDV)抗体的中和(SN)试验、间接荧光抗体技术(IFAT)和间接免疫酶染色法。这3种方法对38份CD弱毒疫苗免疫犬血清抗体效价的测定结果表明,当被检血清稀释度为1∶100时,SN试验、IFAT和间接免疫酶染色法测定时的阳性血清数分别为29,7和31份,IFAT和间接免疫酶染色法测定结果相对于SN试验结果的符合率分别为42.1%和94.7%。同时发现,当SN试验测定的血清效价在1∶100以上时,IFAT测定结果总是在1∶25以上,间接免疫酶染色法测定结果总是在1∶100以上。3种方法以各自初步确定的CDV血清抗体效价完全保护值指标计算所测血清的完全保护率,SN试验为76.3%,IFAT为78.9%,间接免疫酶染色法为81.6%。据此认为,IFAT和间接免疫酶染色法均可部分代替SN试验用于CD疫苗免疫效果的评价、免疫犬抗体水平的监测以及CD的流行病学调查 相似文献
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用抗传染性氏囊病毒单克隆抗体建立夹心阻断ELISA检测鸡血清抗体及 … 总被引:1,自引:0,他引:1
朱红 《动物科学与动物医学》2000,17(5):51-52
用酶标记抗传染性法氏囊病毒(IBDV)单克隆抗体,建立夹心阻断ELISA,检测IBDV鸡血清抗体。用D78细胞毒免疫24日龄的雏鸡,每周采血一次,共4次,用夹心阻断ELISA、微量细胞中和试验(VN)、琼脂扩散试验(NGP)检测鸡血清抗体,结果表明:夹心阻断ELISA同VN之间具有较高的相关性(r=0.8126),与AGP的相关性较低(r=0X.7575)。 相似文献
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A Marek's disease (MD) lymphoblastoid cell line, MDCC-MSB1-41C, was highly transplantable and lethal for chickens. Autopsies showed extensive metastasis in various organs. The transplantabilities of the parent cell line, MDCC-MSB1, and another derivative line, MDCC-MSB1-33C, were transient. MD virus (MDV) could be isolated from the kidneys but not from the peripheral blood leukocytes of chickens inoculated with the MSB1-41C cell line. In addition, anti-MDV antibodies were produced both in chickens inoculated with this cell line and in controls raised with inoculated chickens, but several attempts to isolate MDV from this cell line in vitro failed. 相似文献
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Chuan Yu Qiu Liu Aijian Qin Xuming Hu Wencai Xu Kun Qian Hongxia Shao Wenjie Jin 《Veterinary research communications》2013,37(4):277-283
Marek’s disease virus (MDV) is a highly cell-associated herpesvirus that causes a disease in chickens characterized by tumor formation and immunosuppression. The changes of major histocompatibility complex (MHC) expression in different MDV-infected cells are not completely understood. In this study, we investigated the expression of the Class I MHC and β2-microglobulin (β2m) genes in response to MDV infection at different time points by real-time PCR. In both in vitro and in vivo, the expression levels of Class I MHC and β2m genes were upregulated during early MDV infections in comparison to control cells; We also found that the expression of Class I MHC gene was downregulated in BudR (5-bromo-2′-deoxyuridine)-treated MSB1 cells at 48 h and MDV-infected chicken embryo fibroblast cells (CEF) at 120 and 168 h post infection (hpi); Furthermore, compared to control groups, Class I MHC and β2m expression levels were downregulated in peripheral blood lymphocytes (PBLC) from MDV-infected chickens at 14 and 28 days post infection (dpi); Interestingly, both Class I MHC and β2m gene expression levels increased again in PBLC from MDV RB1B-infected chickens at 35 dpi, in which MDV was in the latent or transformed infection stages. In addition, Class I MHC expression was clearly decreased in MDV-infected CEF at 120 hpi although β2m expression was significantly increased. These changes in Class I MHC and β2m gene expression might provide more insights into host-virus interaction. 相似文献
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鸡贫血病毒VP1和VP2蛋白在家蚕中的联合表达 总被引:1,自引:0,他引:1
将鸡贫血病毒VP1和VP2基因分别克隆入转换载体pBacPAK8中,获得重组转移质粒pBac-vp1和pBac-vp2。以上两质粒分别与CvnⅠ酶切线性化的亲本病毒Bm-BacPAK6DNA共转染家蚕细胞,通过蓝白斑筛选,纯化得到重组病毒Bm-vp1和Bm-vp2。PCR分析表明Vp1和Vp2基因已整合进杆状病毒基因组中。将Bm-vp1和Bm-vp2共感染5龄家蚕,通过表达产物免疫SPF鸡产生的抗血清与CAV感染的MDCC-MSB1细胞的间接荧光抗体分析,证明表达产物能诱导鸡产生相应的抗体。该研究表明,表达VP1和VP2蛋白的重组家蚕杆状病毒(recombinant BmNPV)是很有前途的CAV亚单位疫苗的生产系统。 相似文献
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Diversity (polymorphism) of the meq gene in the attenuated Marek's disease virus (MDV) serotype 1 and MDV-transformed cell lines 总被引:5,自引:0,他引:5
Chang KS Ohashi K Onuma M 《The Journal of veterinary medical science / the Japanese Society of Veterinary Science》2002,64(12):1097-1101
The meq gene encoding a 339-amino-acid bZIP transactivator protein has been identified as a candidate oncogene of Marek's disease virus serotype 1 (MDV1), which induces malignant lymphomas in chickens. We have previously reported that, in addition to meq, L-meq, in which a 180-bp sequence is inserted into the region encoding the transactivation domain of meq, is also detected in chickens experimentally infected with MDV. To further analyze the diversity in meq, PCR was performed using a primer set which specifically amplify the proline-rich repeat (PRR) region in the transactivation domain of meq. In CVI988/R6, a vaccine strain of MDV1, and JM, an MDV1 strain attenuated by prolonged passage in vitro, a major band of a 0.8 kb corresponding to L-meq as well as a minor band of 0.6 kb corresponding to meq was detected by PCR. Furthermore, extra 0.5- and 0.3-kb bands, corresponding to genes termed as short meq (S-meq), and very short meq (VS-meq), respectively, were also detected. These genes were also detected in MDV-transformed cell lines, MSB1 and MTB1. In Md5, an oncogenic MDV1, attenuated by prolonged passage in vitro, the 0.6-kb meq was consistently detected, and 0.5-kb S-meq was occasionally detected. This diversity in meq was due to the difference in the copy number of the PRR region: L-meq and meq contained 9 and 6 copies of PRR while 4 and 2 copies of PRR were present in S-meq and VS-meq, respectively. Thus, the meq gene is polymorphic in the attenuated MDV1 and the MDV-transformed cell lines, and gene products from different meq genes may have different functions from each other. 相似文献
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应用宜兴赛尔生物化工厂产199、F-10、1640和DMEM细胞培养基与美国Sigma公司产199、F-10、1640和DMEM细胞培养基分别配制细胞培养液,培养SP2/0和Vero细胞系及原代鸡胚成纤维细胞(CEF),做细胞培养动力学比较试验。比较这两种来源的细胞培养基对细胞生长的形态、分裂速度及鸡马立克氏病毒(Marek'sdiseasevirus.MDV)疫苗毒株HVT-FC126和RispensCVI988在CEF单层上增殖量的差异。研究结果表明,四种国产细胞培养基与对应的四种进口培养基对细胞生长及病毒增殖的影响无显著差异 相似文献
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根据马立克氏病病毒(MDV)国际参考强毒CA株pp24基因序列,设计和合成了一对引物,其两端分别含SalI和EcoRI的酶切位点,以CV1988株基因组DNA为模板,通过PCR技术,扩增其pp24基因。PCR产物经纯化后,按正确的阅读框架定向克隆到表达性载体pGEX-6P-1中谷胱甘肽转移酶(GST)基因的下游,并用序列测定验证。将重组质粒转化的大肠杆菌BL21,在1.0mMIPTG和37℃条件下诱导,GST-pp24基因获得了表达。诱导菌体的裂解物经12%的SDS聚丙烯凝胶电泳(SDS-PAGE)和Westemblot试验验证。得到大小为43kD的融合蛋白,与预期大小一致。将该融合蛋白的凝胶带切下研碎后免疫小鼠三次后,其血清与MDV感染的鸡胚成纤维细胞(CEF)在间接免疫荧光试验中呈阳性反应。 相似文献
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将人参总皂甙经化学转化成转化型人参皂甙后分离得8个组分,在体外细胞上进行了转化型人参皂甙8个组分对CEF细胞毒性、生长活性、诱导肿瘤细胞凋亡、诱导单克隆抗体生成以及抗IBDV、AIV(H9)、NDV、MDV病毒的活性研究。结果发现,转化型人参皂甙各组分的细胞毒性作用在23.26~39.53mg/L之间;对鸡胚成纤维细胞(CEF)的生长和活性呈促进作用的工作浓度在10~20mg/L之间;转化型人参皂甙8号组分12.5mg/L诱导48h后,肝癌细胞7402株有60%的细胞凋亡,大鼠脑胶质瘤细胞C6株有35%的细胞凋亡;3、4、7号组分12.5mg/L和6.25mg/L对单克隆抗体6E6株杂交瘤细胞和单克隆抗体10B11株杂交瘤细胞的单抗生成具有明显促进作用,其HI效价为2^6~7与对照组的2^5相比有明显差异,IFA效价为10^4~5与对照组的10^2相比有极显著差异;4、7、8号组分15mg/L阻斯IBDV、AIV(H9)、NDV感染CEF细胞的作用都达到了51.1%以上,抑制IBDV、AIV(H9)、NDV在CEF上增殖的作用都在30%以上;6、7号组分12.5mg/L在阻断感染、抑制增殖、直接杀灭3种方式的抗MDV—RB1B强毒株在SPF鸡CEF细胞上的空斑减数率都达了到ACV抗MDV空斑减数率的80%,其中4、6号组分对MDV—RBIB株的直接杀灭作用与ACV的杀灭作用相等。表明人参总皂甙经化学处理转变成转化型人参皂甙,可明显改变其生物学活性。 相似文献