免疫组化、Western blot蛋白印迹和免疫荧光染色观察磷酸鞘氨醇受体2大鼠海马中的表达变化

目的观察磷酸鞘氨醇受体2(S1PR2)基因在颞叶癫痫大鼠海马中的表达变化。方法将72只健康雄性Wistar大鼠随机均分为实验组(36例)和对照组(36例)。实验组使用氯化锂—匹罗卡品进行颞叶癫痫诱导制模,成功后持续大发作1h终止待检,对照组以相同剂量生理盐水注射,然后以进行免疫组化、Western blot印迹和免疫荧光染色检测并进行统计学分析。结果免疫组化检测结果显示,两组1d、3d、7d、28d、56d海马S1PR2阳性细胞计数相比有统计学意义(P<0.05);Western blot检测结果显示,两组3d、7d、28d、56d海马S1PR2蛋白表达水平相比有统计学意义(P<0.05);免疫荧光染色检测显示,S1PR2蛋白表达阳性为红色,星形胶质细胞为绿色,细胞核为蓝色。结论颞叶癫痫大鼠海马中S1PR2表达水平显著下降,说明颞叶癫痫发病机制可能与神经元功能、星形胶质细胞增生受到S1PR2影响有关。

Generation and characterization of an anti-GP73 monoclonal antibody for immunoblotting and sandwich ELISA

Recently, serum Golgi protein 73 （GP73） levels have been found to be elevated in patients with hepatocellu- lar carcinoma （HCC）, and GP73 has been proposed as a novel marker for HCC. However, GP73 levels in patients remain controversial due to the specificity of the anti-GP73 antibody-based enzyme linked immunosorbent as- say （ELISA）. Therefore, an anti-GP73 antibody with high specificity was highly demanded. In the present study, by hybridoma screening, we generated an anti-GP73 monoclonal antibody （mAb） designated as 6A2 using recom- binant GP73 protein produced by prokaryotic expression. The specificity of 6A2 was evaluated by Western blot- ting, immunohistochemistry and immunoprecipitation. The results showed that 6A2 recognized GP73 in both native and denatured forms. In addition, we have developed a sandwich ELISA using 6A2 and GP73 polyclonal antibody generated in New Zealand white rabbits according to standard procedures, and measured the serum GP73 level of patients using this assay. Our results showed that serum GP73 levels of HCC patients were significantly higher than those of healthy controls （P = 0.0036）. Furthermore, for the first time, GP73 serum level was found to be elevated in patients with breast cancer compared with healthy controls （P = 0.0172）.

一个Western Blot与DNA电泳定量自动分析系统

针对Western Blot以及DNA电泳等实验研究结果定量分析主要应用凝胶成像系统完成,定量分析软件操作流程繁琐的特点,设计出一个适用于Western Blot及DNA电泳等结果定量分析系统。介绍系统中图像处理的问题:图像二值化、分割与感兴趣区域提取、定量分析中的面积计算,着重从计算机图像处理的角度说明定量分析的解决方案。实验证明,系统能够减少实验员人工干预操作,定量分析结果能够满足Western Blot及DNA电泳等实验研究定量分析的应用需要。

Interpretation Criteria for Standardized Western Blot for the Predominant Species of Borrelia Burgdorferi Sensu Lato in China

Objective Western blotting （WB;immunoblotting） is a widely used tool for the serodiagnosis of Lyme borreliosis （LB）,but so far,no generally accepted criteria for its performance and interpretation have been established in China.The present study was designed to determine the criteria for standardized Western blot for the predominant species of Borrelia burgdorferi sensu lato in China,in which WB was produced with strain PD91 as the representative strain attributed to predominant genospecies Borrelia garinii of Borrelia burgdorferi sensu lato.Methods Approximately 13 bands between 14 and 100 kD were differentiated for strain PD91 by using Gel-Pro analysis software.In a study with 631 serum samples （taken from 127 patients with Lyme borreliosis and 504 controls）,all observed bands were documented.To establish criteria for a positive WB result for strain PD91,receiver operating characteristic （ROC） curves were used.Results The following interpretation criteria were recommended：for IgG,at least one band of P83/100,P58,P39,P30,OspC,P17,P66,and OspA;for IgM,at least one band of P83/100,P58,OspA,P30,OspC,P17 or P41.In addition,syphilis,leptospirosis and other related diseases should be excluded when the positive band is P41 in IgM.For IgG criteria,the sensitivity is 73.2%,the specificity is 99.4% and Youden index is 0.726;for IgM criteria,the sensitivity is 50.6%,the specificity is 93.1% and Youden index is 0.437.Conclusion Standardization of WB assays is necessary for comparison of results from different laboratories.Moreover,the criteria of other genospecies of Borrelia burgdorferi sensu lato should be determined in the future to complete the criteria of WB for the diagnosis of the Lyme disease in China.

A Study of the Technique of Western Blot for Diagnosis of Lyme Disease caused by Borrelia afzelii in China

Objective To study the technique of Western blot for the diagnosis of Lyme disease caused by Borrelia afzelii in China and to establish the standard criteria by operational procedure. Methods FP1, which is the representative strain of B. afzelii in China, was analyzed by SDS-PAGE, electro transfer and irnmunoblotting assays. The molecular weights of the protein bands of FP1 were analyzed by Gel-Pro analysis software. In a study using 451 serum samples （159 patients with Lyme disease and 292 controls）, all observed bands were recorded. The accuracy of the WB as a diagnostic test was established by using the ROC curve and Youden index. Results Criteria for a positive diagnosis of Lyme disease were established as at least one band of P83/100, P58, P39, OspB, OspA, P30, P28, OspC, P17, and P14 in the IgG test and at least one band of P83/100, P58, P39, OspA, P30, P28, OspC, P17, and P41 in the IgM test. For IgG criteria, the sensitivity, specificity and Youden index were 69.8%, 98.3%, and 0.681, respectively; for IgM criteria, the sensitivity, specificity and Youden index were 47%, 94.2%, and 0.412, respectively.

Analysis of Protoscoleces-specific Antigens from Echinococcus Granulosus with Proteomics Combined with Western Blot

Objective To establish and optimize the proteomic analysis of protoscoleces-specific antigens from Echinococcus granulosus. To provide a foundation for identifying specific antigens in the soluble proteins of E. granulosus protoscoleces for further research. Methods Brood capsules were collected aseptically from fertile E. granulosus cysts from the livers of an infected patient. The fertile E. granulosus cysts were fractured, and protoscoleces were collected by centrifugation. The soluble proteins of protoscoleces were acquired using the 2D Quant kit according to the manufacturer＇s instructions. We employed two-dimensional electrophoresis （2-DE） combined with immunoblot assay （Western blot） to analyze the soluble components of E. granulosus protoscoleces antigens. The 2-DE and immunoblot maps obtained were analyzed with PDQuest 8.0 image analysis software. Results About 233 soluble protein spots were identified with Coomassie-stained gels. Most of the proteins had a molecular weight of 16 000 Da to 117 000 Da, and an isoelectric point value of 3.0 to 10.0. 2-DE immunoblot was conducted and 57 specific antigen spots were observed, among which 23 spots were identified. Conclusion 2-DE combined with Western blot is the key to successful proteomic analysis and presents a new possibility for searching the specific E. granulosus protoscoleces antigens.

Western blot detection of PMI protein in transgenic rice

Phosphomannose isomerase （PMI） encoding gene manA is a desirable selective marker in transgenic research. Under- standing of its expression patterns in transgenic plant and establishing highly sensitive detection method based on immunoassay have great impacts on the application of PMI. In this study, PMI-specific monoclonal antibodies were generated using recombinant protein as immunogen, and could be used in Western blot to detect as little as 0.5 ng His-tagged PMI protein or rice expressed PMI protein in sample accounted for 0.4% of single rice grain （about 0.08 mg）. PMI protein driven by CaMV-35S promoter was detected in dozens of tested tissues, including root, stem, leaf, panicle, and seed at all developmental stages during rice growing, and PMI protein accounted for about 0.036% of total protein in the leaves at seedling stage. The established method potentially can be used to monitor PMI protein in rice grains.

Detection of H pylori infection by ELISA and Western blot techniques and evaluation of anti CagA seropositivity in adult Turkish dyspeptic patients

AIM: To detect H pylori infection and to evaluate the anti CagA seropositivity in adult Turkish dyspeptic patients. METHODS: We evaluated anti-H pylori IgA, IgG and anti-CagA antibodies using commercial enzyme-linked immunoassay (ELISA) and Western blot in dyspeptic Turkish patients. H pylori status was determined by histology and rapid urease testing. RESULTS: Fifty-six patients were entered. Forty-eight (85.7%) out of the 56 patients were positive for H pylori. H pylori IgG seropositivity was 82.1%, IgA seropositivity 48.2%. CagA ELISA showed that IgG was positive in 50% and IgA in 30.4% of those with H pylori infections. Western blot showed that IgG seropositivity was 80.4% and IgA seropositivity 33.9%. Western blot detected IgG antibodies with reactivity to CagA in 50%, VacA in 62.5%, UreB in 87.5%, UreA in 80.4%, and OMP in 57.1%. None of the tests had a sensitivity and specifi city above 80%. CONCLUSION: None of these commercial tests seems clinically useful for H pylori detection in adult dyspeptic patients, while Western blot can give seropositivity and determine anti-CagA, VacA virulence factor status of Turkish dyspeptic patients in the Izmir region.

基于网络药理学和大鼠体内验证的藏药红景天改善脑微循环障碍作用机制研究

目的基于文献研究、网络药理学、分子对接与实验验证的方法,探究藏药红景天改善脑微循环障碍的核心靶点、关键成分和作用机制。方法通过文献和数据库收集红景天化学成分,利用反向药效团匹配预测红景天的潜在靶点;获取脑微循环障碍靶点,并与红景天靶点映射,构建交集靶点蛋白互作网络,获取核心靶点;构建“中药-成分-核心靶点-疾病”调控网络并获取关键成分;进行GO和KEGG富集分析,构建“核心靶点-信号通路-生物过程”网络;进行分子对接验证;采用RT-qPCR和Western blot进行动物实验验证,进一步证实网络药理学分析结果。结果从红景天中筛选出76个活性成分和285个靶点,获取脑微循环障碍靶点1074个,交集靶点97个,核心靶点6个,关键成分6个。分子对接结果表明,有3个关键成分与核心靶点的结合性大于核心靶点蛋白与其原始配体结合性。RT-qPCR结果显示红景天能下调核心靶点CASP3、AKT1 mRNA水平,Western blot检测结果显示藏药红景天能降低CASP3、AKT1蛋白表达(P<0.05)。结论藏药红景天可通过多成分、多靶点、多通路协同改善脑微循环障碍,该研究为临床应用藏药红景天治疗脑微循环障碍提供实验依据。

Expression of Elk-1 in Non-Small Cell Lung Cancer Detected by Western Blot and Tissue Microarray

Objective： The aim of this study was to investigate the Elk-1 （Ets like transcription factor-1） expression in non-small cell lung cancer （NSCLC） and normal lung tissues and the relationship between its expression and clinicopathological characters. Methods： To observe Elk-1 expression, western blot and immunochemistry （IHC） on tissue microarray （TMA） containing 118 lung cancers and their corresponding normal tissues were used. Results： In western blot and IHC on TMA, Elk-1 was highly expressed in NSCLC, while its expression was almost undetectable in normal lung tissues. Elk- 1 expression in NSCLC had no relationship with the patients＇ age, gender, smoking status and histological type, but had relationship with the differentiation degree, clinical stages and lymphonode metastasis. The expression was lower in early stage group （Ⅰ＋Ⅱ） than in advanced stage group （Ⅲ）, and lower in well-moderately differentiated group than in poorly differentiated group. The same trend was seen with lymphonode metastasis. Conclusion： The progression of NSCLC may be related with the increased Elk-1 expression, and Elk-1 may be regarded as a prognostic factor for NSCLC tissues.

Comparison of indirect immunofluorescence and western blot method in the diagnosis of hantavirus infections

BACKGROUND Serologic cross-reactivity between hantaviruses often complicates the interpretation of the results.AIM To analyze the diagnostic value of indirect immunofluorescence assay(IFA)and western blot(WB)in the diagnosis of hantavirus infections.METHODS One hundred eighty-eight serum samples from Puumala(PUUV)and Dobrava(DOBV)orthohantavirus infected patients were analyzed.Serology was performed using commercial tests(Euroimmun,Lübeck,Germany).RESULTS Using IFA,49.5%of acute-phase samples showed a monotypic response to PUUV,while 50.5% cross-reacted with other hantaviruses.The overall cross-reactivity was higher for immunoglobulin G(IgG)(50.0%)than for immunoglobulin M(IgM)(25.5%).PUUV IgM/IgG antibodies showed low/moderate reactivity with orthohantaviruses Hantaan(12.3%/31.5%),Seoul(7.5%/17.8%),DOBV(5.4%/28.1%),and Saaremaa(4.8%/15.7%).Both DOBV IgM and IgG antibodies were broadly reactive with Hantaan(76.2%/95.2%),Saaremaa(80.9%/83.3%),and Seoul(78.6%/85.7%)and moderate with PUUV(28.5%/38.1%).Using a WB,serotyping was successful in most cross-reactive samples(89.5%).CONCLUSION The presented results indicate that WB is more specific than IFA in the diagnosis of hantavirus infections,confirming serotype in most IFA cross-reactive samples.

以结果验证为导向的中医学八年制Western Blot实践教学

“实验中医学”是海军军区大学中医学八年制学员的主干课程。其中Western Blot是研究蛋白水平的基本方法,也是学员所必须掌握的实验研究方法。本课程以结果验证为导向的教学方式革新,最大限度压缩每个步骤的操作时间,聚焦于让学员完成最多的实验步骤,力求实验的完整性。该方法可在一堂课完成实验,展示结果并进行分析讨论。该教学方式有助于在最短时间内掌握完整的Western Blot实验技术,值得进一步推广应用。

基于特征多肽抗原的阿胶基原鉴定

目的 以特征多肽为半抗原并制备多克隆抗体,鉴定阿胶原材料基原。方法 经文献调研及数据库比对筛选特征多肽,将多肽抗原与血蓝蛋白偶联并免疫Balb/c小鼠制备多克隆抗体,通过ELISA、dot blot和Western blot分析与验证多克隆抗体的产生、效价及特异性。结果 筛选所得5个特征多肽序列均具有T细胞表位和B细胞表位,亲水性-1~0,二级结构大多为无规则卷曲。多肽抗原ECS1、ECS3~ECS5在二次加强免疫后,效价分别为1∶6 400、1∶400、1∶12 800和1∶800。制备所得的多克隆抗体之间不产生交叉反应,而且多克隆抗体Ab-ECS3与驴皮及其伪品蛋白的结合显现出较大差异。结论 以特征多肽为半抗原制备所得的多克隆抗体可通过Western blot对驴皮进行真伪鉴别,为胶类中药的基原鉴定提供了参考。

CREB1和CREB3在胃癌及癌前病变组织中的表达及其临床意义

目的探究环磷腺苷反应元件结合蛋白1(CREB1)和环磷腺苷反应元件结合蛋白3(CREB3)在胃癌及癌前病变组织中的表达及临床意义。方法收集慢性浅表性胃炎40例,慢性萎缩性胃炎伴肠化生40例,异型增生40例,胃癌50例,采用免疫组化法检测CREB1和CREB3在四种组织中的表达,并分析其与临床病理参数的关系。另收集同期新鲜组织慢性浅表性胃炎、慢性萎缩性胃炎伴肠化生、胃癌共30例,应用蛋白印迹法(Western blot)检测CREB1和CREB3在不同胃组织中的表达。利用Kaplan-Meier plotter分析CREB1和CREB3的表达与胃癌患者总生存时间(OS)和无进展生存时间(FP)的相关性。利用STRING数据库分析CREB1和CREB3在信号通路中的位置以及与之相关的上下游基因。结果免疫组化显示:胃癌组、异型增生组、萎缩性胃炎伴肠化生组CREB1、CREB3阳性表达率明显高于慢性浅表性胃炎组(P<0.05);并且CREB1、CREB3在胃癌组的阳性表达率明显高于慢性萎缩性胃炎伴肠化生组(P<0.05),但与异型增生组无统计学差异(P>0.05)。临床病理参数分析得出两者表达水平与浸润深度、TNM分期、脉管侵犯、淋巴结转移相关(P<0.05);与患者性别、年龄、肿瘤大小、分化程度无明显相关性(P>0.05)。Western blot结果显示:CREB1、CREB3蛋白表达在慢性浅表性胃炎、慢性萎缩性胃炎伴肠化生、胃癌中依次增高,差异有统计学意义(P<0.01)。Kaplan-Meier plotter分析显示CREB1、CREB3高表达的胃癌患者OS和FP均缩短。结论CREB1、CREB3可能与胃癌的发生、发展与转移相关,且蛋白高表达可能与胃癌患者预后不良有关。

SIRT6在胃癌中的表达及临床意义

目的探讨沉默信息调节因子6(Sirtuin 6,SIRT6)在胃癌组织中的表达及临床意义。方法生物信息学分析SIRT6 mRNA在胃癌中的表达及其与生存、肿瘤突变负荷(TMB)及TIDE评分的关系;收集95例胃癌及癌旁组织标本,免疫组织化学方法检测SIRT6的表达水平,分析其与临床病理特征的关系;Western blot法检测10例新鲜胃癌及癌旁组织中SIRT6的表达情况。结果生物信息学分析显示,SIRT6 mRNA在胃癌中表达高于正常胃组织(P<0.05),Kaplan-Meier生存曲线显示SIRT6高表达组生存时间较短,突变相关分析及TIDE评分显示SIRT6高表达组具有更高的TMB及TIDE评分(P<0.05),且SIRT6 mRNA表达水平与TMB及TIDE评分呈显著正相关(P<0.05)。免疫组织化学结果显示SIRT6在胃癌组织中表达率为85.2%(81/95);SIRT6在胃癌中高表达与高Ki-67增殖指数相关,差异具有统计学意义(P<0.05),SIRT6表达在不同年龄、性别、肿瘤直径及P53等组间差异均无统计学意义(P>0.05);Western blot显示胃癌组织中SIRT6的表达水平高于癌旁组织(9/10),差异具有统计学意义(P<0.05)。结论SIRT6在胃癌组织中高表达,可能通过影响基因组稳定性及胃癌细胞增殖能力参与胃癌的发生发展。

髓系特异性Spi1基因敲除小鼠的构建和基因鉴定

目的构建髓系特异性Spi1基因敲除小鼠并分析其基因型,为疾病病理机制及药物靶点研究提供动物模型基础。方法根据CRISPR/Cas9技术原理和Cre/LoxP系统,设计并构建sgRNA和Donor载体,以第2号外显子(Exon 2)所在的转录本为敲除区域,在Exon 2两侧各放置同向Loxp元件;将Cas9蛋白、sgRNA和Donor载体混合显微注射到C57BL/6J小鼠的受精卵中,移植受精卵到假孕的C57BL/6J母鼠的子宫中,19~20 d后获得F0代。将阳性F0代小鼠与C57BL/6J小鼠交配,得到稳定的F1代Spi1^(flox/+)小鼠。F1代Spi1^(flox/+)小鼠雌雄自交得到Spi1^(flox/flox)小鼠。Spi1^(flox/flox)与Lyz2-Cre^(+)小鼠交配得到Spi1^(flox/+)/Lyz2-Cre^(+)小鼠,再将其与Spi1^(flox/flox)交配,得到的Spi1^(flox/flox)/Lyz2-Cre^(+)小鼠为髓系特异性Spi1基因敲除(KO)小鼠;Spi1^(flox/flox)/Lyz2-Cre^(-)小鼠作为野生型(WT)小鼠。提取WT和KO小鼠DNA,PCR扩增后琼脂糖凝胶电泳鉴定基因型;Western blot检测WT和KO小鼠免疫细胞中脾病灶形成病毒前病毒整合癌基因-1/富含嘌呤盒1(PU.1)表达。结果PCR鉴定结果显示,采用flox引物鉴定时仅扩增出220 bp条带的小鼠,即基因型为Spi1^(flox/flox)纯合子,采用Lyz2-Cre引物鉴定时扩增出700 bp的小鼠,基因型为Lyz2-Cre^(+);Western blot结果显示,与WT组比较,KO组小鼠骨髓来源巨噬细胞(BMDMs)和腹腔原位巨噬细胞(PM)中的PU.1不表达(P<0.01);T细胞中KO小鼠PU.1表达水平与WT小鼠差异无统计学意义;PCR和Western blot结果均表明髓系特异性Spi1 KO小鼠构建成功。结论成功构建和鉴定髓系特异性Spi1 KO小鼠,为进一步揭示PU.1在免疫调节中的潜在机制研究提供动物模型基础。

甘草总黄酮对高脂条件下罗非鱼肝损伤的保护作用

为了研究甘草总黄酮对高脂饲料造成的罗非鱼(Oreochromis niloticus)脂肪肝损伤是否具有保护作用,随机将180尾健康无伤罗非鱼分成6组,即对照组、高脂饲料模型组和4个不同浓度甘草总黄酮组(0.05、0.10、0.50、1.00 g·kg^(-1)甘草总黄酮),每组30尾。饲喂90 d后,采集罗非鱼各实验组肝,测定肝匀浆中超氧化物歧化酶(SOD)活性、还原型谷胱甘肽(GSH)活性、丙二醛(MDA)含量、甘油三酯(TG)含量、总胆固醇(TC)含量、总抗氧化能力(T-AOC)水平,Western blotting法检测肝中核转录因子-κB P65(NF-κB P65)和核转录因子-κB C-Rel(NF-κB C-Rel)蛋白表达水平,RT-PCR法测定肝中微粒体甘油三酸酯转移蛋白(MTTP)和载脂蛋白B100(ApoB100)基因表达情况。结果表明:与对照组相比,高脂饲料模型组罗非鱼肝匀浆中TG、TC、MDA含量极显著(P<0.01)升高,GSH活性、SOD活性、T-AOC水平均极显著(P<0.01)降低;MTTP和ApoB100 mRNA表达水平降低(P<0.01或P<0.05);Western blotting结果显示,NF-κB P 65和C-Rel蛋白表达水平升高。饲料中加入甘草总黄酮后,与高脂饲料模型组相比,罗非鱼肝中GSH活性、SOD活性、T-AOC水平不同程度提高,TC、TG、MDA含量和NF-κB P65、C-Rel蛋白表达水平不同程度降低,MTTP和ApoB100的mRNA表达水平升高,以0.50 g·kg^(-1)甘草总黄酮组效果较好。说明甘草总黄酮对于罗非鱼脂肪肝损伤具有一定的保护作用,可以缓解高脂饲料造成的脂肪肝损伤。

肝硬化大鼠肾组织变化及血红素加氧酶-1的表达

目的探讨实验性肝硬化大鼠肾脏病理组织学改变及其血红素加氧酶-1(heme oxygenase-1,HO-1)在大鼠肾组织中的表达变化。方法通过胆总管结扎术(common bile duct ligation,CBDL)建立胆汁性肝硬化大鼠模型。将30只SD大鼠随机分为3组:假手术组(SO组)、CBDL术后2周组和CBDL术后5周组。观察实验大鼠肝脏、肾脏组织病理学改变,测定肝硬化大鼠内生肌酐清除率(creatinine clearance rate,CCR)和丙二醛(malondialdehyde,MDA)含量。应用TUNEL法检测肝硬化大鼠肾组织细胞的凋亡率,免疫组化和Western blotting检测HO-1在肝硬化大鼠肾组织细胞中的表达。结果CBDL大鼠模型2周时肝脏出现纤维化,5周时形成肝硬化。5周时,光镜下肾小管上皮细胞坏死脱落;电镜下示足突细胞广泛融合,细胞数减少,肾间质系膜区变宽,毛细血管基底膜不规则增厚。CBDL大鼠在2周和5周时CCR逐渐降低(P<0.05),肾组织MDA含量升高(P<0.01)。实验大鼠肾组织细胞凋亡率于5周时达到高峰,肾组织细胞HO-1阳性表达率则最低,与2周时比较,差异有统计学意义(P<0.05)。Person相关分析显示,实验大鼠肾组织MDA与凋亡率呈正相关,肾组织HO-1表达与细胞凋亡率呈负相关,差异均有统计学意义(P<0.05)。结论胆汁性肝硬化大鼠肾脏存在病理组织学改变,HO-1参与了大鼠肾组织损伤的病理生理过程。

复方中草药对运输后肉牛应激蛋白mRNA和蛋白表达水平的影响

文章旨在研究复方中草药对运输后肉牛应激蛋白mRNA和蛋白表达水平的影响,试验将40头健康、体重相近的荷斯坦育肥牛随机分成4组,每组10个重复,分别为对照组(1组)、0.5%(2组)、1.0%(3组)、1.5%(4组)复方中草药添加组,饲喂14 d后模拟运输应激。采用ELISA测定运输前、后荷斯坦育肥牛血清中HSP 70含量,采用荧光定量PCR(qRT-PCR)和Western Blotting分别测定运输后组织中HSP 70、HSP 90及HSP 27的mRNA和蛋白质水平的表达量。结果显示,运输后的各组荷斯坦育肥牛血清中HSP 70含量均高于运输前的(P<0.05),与对照组相比,试验3、4组试验运输前和运输后荷斯坦育肥牛血清中HSP 70含量显著降低(P<0.05),试验3、4组运输后的肉牛肌肉组织HSP 27、HSP 70及HSP 90的mRNA的表达量显著降低(P<0.05);试验3、4组运输后的肉牛肌肉组织HSP 70和HSP 90蛋白表达量显著降低(P<0.05)。说明运输可以提高肉牛血清和肌肉组织中应激蛋白含量,添加不同水平的复方中草药可以降低运输后肉牛血清及肌肉组织中应激蛋白的水平,以添加量为1.0%较适宜。

血清4型禽腺病毒Fiber-2蛋白截短表达及单克隆抗体制备

【目的】获得截短表达的血清4型禽腺病毒(FAdV-4)Fiber-2重组蛋白及其单克隆抗体,为建立快速灵敏的病毒检测方法提供基础材料。【方法】对Fiber-2基因序列进行密码子优化,截取Fiber-2蛋白抗原性集中片段,PCR扩增其基因序列,连接至pET-32a(+)构建原核表达载体。将表达的重组蛋白进行纯化,并通过Western blotting验证其在大肠杆菌中的表达情况。将重组蛋白免疫BALB/c小鼠后取脾细胞与SP2/0细胞融合,利用间接酶联免疫吸附试验(ELISA)法筛选阳性细胞株,再利用秋水仙素裂解法、间接ELISA法和间接免疫荧光法(IFA)对其进行鉴定。【结果】成功构建Fiber-2基因截短片段的原核表达系统,获得大小约为67 kD的Fiber-2截短蛋白,以包涵体的形式出现,经纯化后可获得单一的特异性条带,经Western blotting鉴定证明其可与FAdV-4阳性血清结合从而产生一条特异性条带。经过4次亚克隆后筛选到5株能稳定分泌抗体的杂交瘤细胞株(2C2、4F6、5A5、6G10和10B5),其抗体分泌稳定性、特异性好,诱生的细胞上清液抗体效价为1:1600~1:6400,腹水抗体效价为1:320000~1:1280000,秋水仙素裂解检测染色体数目为94~110条。2C2、4F6和10B5杂交瘤细胞分泌的抗体重链为IgG2b亚型,轻链为Kappa链;5A5和6G10杂交瘤细胞分泌的抗体重链为IgG1亚型,轻链为Kappa链。5株杂交瘤细胞株与感染FAdV-4的鸡肝癌上皮细胞系(LMH)进行IFA检测,结果均为阳性。【结论】制备的Fiber-2截短重组蛋白及单克隆抗体具有良好的反应原性和特异性,可用于FAdV-4病毒检测试剂盒研发。