新疆生鲜乳质量安全发展现状及存在的问题

阐述了新疆生鲜乳生产现状，发现乳产业中存在的质量安全问题，并在此基础上对国内外生鲜乳质量安全研究现状进行分析，对现有生鲜乳质量安全检测技术进行介绍，期望能为新疆生鲜乳行业的健康快速发展提供一定的帮助。      

The M43 domain-containing metalloprotease RcMEP1 in Rhizoctonia cerealis is a pathogenicity factor during the fungus infection to wheat

Wheat(Triticum aestivum L.) is an important staple crop for global human. The necrotrophic fungus Rhizoctonia cerealis is the causal pathogen of sharp eyespot, a devastating disease of wheat. Herein, we identified RcMEP1, a zinc metalloproteaseencoding gene from R. cerealis genomic sequences, and characterized its pathogenesis function. RcMEP1 expressed at markedly-high levels during R. cerealis infection process to wheat. The predicted protein RcMEP1 comprises of 287 amino acid residues and contains a signal peptide and a M43 metalloprotease domain harboring the active site motif(HEVGHWLGLYH). The assays of Agrobacterium tumefaciens-mediated transient expression in Nicotiana benthamiana leaves indicated that RcMEP1 is an apoplastic elicitor of cell death, and that the predicted signal peptide functions and is required for secretion and cell death-induction. The purified RcMEP1 protein and its M43 domain peptide were individually able to induce plant cell death and H2 O2 accumulation, and to inhibit expression of host chitinases when infiltrated into wheat and N. benthamiana leaves, while the M43 domain-deleting peptide and negative control lacked the capacity. Moreover, compared with the control pretreatment, the purified RcMEP1 protein or its M43-domain peptide resulted in enhanced pathogenesis in the inoculated wheat, whereas the M43 domain-deleting peptide failed. These results suggest that RcMEP1 acted as an important pathogenicity factor during R. cerealis infection to wheat and that its signal peptide and M43 domain are required for the secretion and pathogenesis of RcMEP1. This study provides insights into pathogenesis role of M43 domain-containing metalloproteases during R. cerealis infection to wheat.     

牦牛病毒性腹泻/粘膜病的防制研究

20世纪80年代以来，我国牦牛群中陆续发现牛病毒性腹泻／粘膜病(BVD／MD)，血清阳性率在30％～42．4％之间，病死率在30％左右，本研究先后从四川、西藏等地牦牛中分离出病毒，并对其进行各种生物学特征鉴定后，表明该病毒与标准毒属同一种，所不同的是四川牦牛病毒株属非致细胞病变型，即属NCP型。但回归本动物能复制出典型病例。目前尚无国产牛粘膜病疫苗用于生产。本研究依据猪瘟病毒与牛病毒性腹泻／粘膜病病毒具有交叉免疫性的原理，用猪瘟弱毒苗对牦牛病毒性腹泻／粘膜病进行预防，试验证明用猪瘟弱毒苗可以预防牛病毒性腹泻／粘膜病，且安全可靠，具有实用价值。     

优质啤酒大麦品种比较试验结果初报

2003年在古浪县良种场进行的5个啤酒大麦品种品比试验结果表明,B1202折合产量最高,为8510kg/hm2,较对照品种法瓦维特增产17.6%,可作为主栽品种;甘啤3号较对照法瓦维特增产4.8%,可作为搭配品种。B1614、B4947、哈林顿3个品种较对照品种减产8.7%～25.7%,可淘汰。     

转译过程中小RNA病毒与宿主细胞的相互作用

小RNA病毒的转译机制不同于真核细胞mRNA的转译机制,该类病毒是借助于内部核糖体进入位点来启动内部翻译过程的,同时还伴随着宿主细胞蛋白质合成的抑制过程.在此过程中,小RNA病毒与宿主细胞间发生了一系列复杂的相互作用和信息交流,本文对该领域的研究进展作了综述.     

猪传染性胃肠炎病毒南京株纤突S蛋白基因的克隆与序列分析

参考 Genbank收录的 TGEV- Miller株的基因序列 ,自行设计合成 1对引物 (TGEVP5 /P6 ) ,对不同代次的 TGEV疫苗弱毒 STC3及种毒 、种毒 进行了 RT- PCR扩增 ,产物经琼脂糖凝胶电泳分析 ,均出现 1条大约 12 6 2 bp的目的条带 ,经 Eco R 酶切 ,都产生了 871bp和391bp左右的两个片段 ,与预期大小相符。将种毒 RT- PCR扩增目的条带回收纯化后克隆入PMD18- T载体中 ,转化宿主菌 DH5 α,挑选阳性克隆 (命名为 PTs) ,提取重组质粒 ,用 Hpa 、Eco R 对重组质粒进行酶切鉴定以及 PCR扩增 ,然后进行序列测定 ,并进行了序列分析 ,证实与国外标准毒株 Miller、Fs772 / 70、Purdue、TO14等有较高的同源性     

白花柽柳nrDNA的ITS序列片段研究

运用PCR直接测序法 ,对白花柽柳 (TamarixalbiflonumM .T .Liu .)的nrDNA的ITS区 (包括ITS -l,5 .8SrDNA和ITS - 2 )进行序列测定。结果表明 ,该植物的ITS序列和长穗柽柳 (Tamarixelongata)的序列差别不大 :ITS - 1片段的长度都是 2 5 9bp ;ITS - 2片段的长度同为 2 44bp ;G C百分含量仅相差 1% ;碱基差异共发生 18处。由ITS及 5 .8SrDNA序列分子证据看 ,白花柽柳更可能是长穗柽柳的变异。     

Analysis of the distribution and clonality of TCR Vβ T cells in cord blood

AIM:To investigate the distribution and clonality of TCR Vβ subfamily T cells in cord blood. METHODS:The CDR3 of TCR Vβ 24 subfamily genes were amplified in mononuclear cells from 13 cases of cord blood. To observe the usage of TCR Vβ repertoire, the PCR products were further labeled with fluorescent and analyzed by genescan technique for the CDR3 size, to evaluate clonality of the detectable TCR Vβ T cells. Peripheral bloods from 10 cases of normal individuals and T cell line Molt-4 and Jurkat served as controls. RESULTS:Only 38.78%±16.26% of 24 Vβ subfamily T cell were selectively expressed in cord blood, predominantly in Vβ 3, 5, 8, 9 and 13, whereas all 24 Vβ subfamilies could be detected in T cells from peripheral blood of normal individuals. Genescan analysis showed that all PCR products of TCR Vβ subfamilies from cord blood or normal individual peripheral blood displayed multi-peaks. CONCLUSION:Some TCR Vβ subfamily T cells were absent in cord blood. All TCR Vβ subfamily T cells in cord blood displayed polyclonality.     

奶牛MTT比色法的最佳条件探讨

为建立奶牛淋巴细胞增殖反应MTT比色法,对试验条件进行了研究。应用L16(45)正交试验,对影响MTT比色法的四个主要因素,包括ConA浓度、细胞浓度、培养液小牛血清浓度及培养时间进行了比较和探索。试验表明几个因素对其增殖反应都有显著影响(P<0.05),且最佳反应条件为:15μg/mL的ConA、1×106/mL细胞浓度、10%小牛血清及60h的培养时间;影响增殖反应的先后顺序为细胞浓度、ConA浓度、培养时间及血清浓度。