Glycosylation-independent binding to extracellular domains 11-13 of mannose-6-phosphate/insulin-like growth factor-2 receptor mediates the effects of soluble CREG on the phenotypic proliferation of vascular smooth muscle cells

Background The present study aimed to investigate the detailed mode and specific sites for their binding as well as the functional relevance of this binding in the phenotypic proliferation of vascular smooth muscle cells(SMCs). Methods CREG knocked-down SMCs were employed to evaluate the biological activity of wtCREG and mCREG.Expressions of SMC differentiation markers SM myosin heavy chain(SM-MHC),SM-actin,heavy caldesmon and myocardin were determined by Western blotting using specific antibodies. Cellular growth of SMCs was assessed by bromide dewuridine (BrdU) incorporation and cell cycle analysis on fluorescence-activated cell sorting(FACS).A solid-phase binding assay was used to study the binding of CREG to extracellular domains of M6P/IGF2R.The cellular co-localization of the two recombinant CREGs with M6P/IGF2R was detected on SMC surface by immunoprecipitation and immunofluorescence analysis.Results The molecular weight of wtCREG was around 30 kD while that of the mCREG was～25 kD.Treatment of wtCREG with PNGase F reduced its molecular weight from～30 kD to～25 kD,whereas PNGase F treatment had no effect on the molecular weight of mCREG.Both wtCREG and mCREG proteins enhanced SMC differentiation,inhibited BrdU incorporation,and arrested cell cycle progression when added to the culture medium.In CREG knocked-down SMCs,the amount of CREG detected by immunoblotting in M6P/IGF2R immunoprecipitates was significantly reduced when compared to normal cells.Both recombinant CREGs co-immunoprecipitated with M6P/IGF2R, although slightly reduced amount of the mutant CREG was detected in M6P/IGF2R immunoprecipitates.Immunostaining revealed that His-tagged CREGs co-localized with IGF2R on the cell surface in a glycosylation-independent manner.In vitro binding assay showed that CREGs bound to M6P/ IGF2R extracellular domains 7-10 and 11-13 in a glycosylation -dependent and -independent manner,respectively.Further blocking experiments using soluble M6P/IGF2R fragments and M6P/IGF2R neutralizing antibody indicated that the biological activities of recombinant CREGs in SMC growth and the up-regulation of SMC differentiation markers were all abolished by treatment with the M6P/IGF2R neutralizing antibody. However,although the growth inhibitory effect of wtCREG was nearly abolished by D7-10 or D11-13,the effect of mCREG was only reversed by Dll-13,indicating that the binding to domains 11-13 is required for CREG to modulate the proliferation of SMCs.Conclusions These data suggest that solubleCREG proteins can exert their biological function via binding to the extracellular domains 7-10 and 11-13 of cell surface M6P/IGF2R in both a glycosylation-dependent and -independent manner.

Enhanced immuno-detection of shed extracellular domain of HER-2/neu

HER-2/neu oncogene is over-expressed and amplified in patients associated with metastatic breast cancer. An increased level (>15 ng/mL) in the shed extracellular domain (sECD-HER 2/neu) is indicative of the potential presence and as-sociated progression of this disease. A fluo-rescent ELISA incorporating the newly devel-oped ALYGNSA antibody-orientation system revealed a 10-fold increase in sensitivity (≤0.63 ng/mL) of sECD-HER 2/neu when compared to a control standard ELISA kit (≤7.5 ng/mL). This enhanced mode of detection has the potential to not only address breast and other cancers per se but also permit an in depth evaluation of “shed extracellular domains”, in general, and the role of these “proteolytic derived factors” in physiological signalling at normal levels.

Eukaryotic expression, purification and activity characterization of human soluble DSG2 extracellular domain protein

Objective:To construct a secretory eukaryotic expression vector of DSG2 fused with the Fc region of the human IgG,to validate its expression in 293T cells,and to purify the secretory protein with biological activity.Methods:The DSG2 extracellular domain fragment gene(DSG2ex),was amplified by PCR,and was inserted into the eukaryotic expression plasmid pCMV3-IgG1 to construct the recombinant eukaryotic expression plasmid-pCMV3-DSG2ex-IgG1.The successfully constructed eukaryotic expression plasmid was transfected into 293T cells to express and secrete DSG2 extracellular domain protein.The targeted protein was purified from the cell culture supernatant by Protein A affinity chromatography and confirmed by Western Blotting and ELISA.Results:The pCMV3-DSG2ex-IgG1 eukaryotic expression plasmid was successfully constructed.The highest protein expression level was obtained with 293T cells after 96 h of transfection.The relative molecular mass of the purified product was between 100 and 130 kDa was estimated by SDS-PAGE,which was consistent with the expectation.The yield of the purified protein reached 0.8 mg/ml with a purity over 90%.The purified DSG2 extracellular domain protein with IgG1 tag was recognized by IgG monoclonal antibodies by Western blotting.Moreover,the ELISA results showed that the prepared DSG2 extracellular domain protein had significant binding activity to human type 55 adenovirus Fiber Knob protein(HAdV-55).Conclusion:A simple and efficient method for eukaryotic expression and purification of human soluble DSG2 extracellular domain protein was successfully established,and biologically active DSG2 extracellular domain protein was purified,which laid the foundation for the later study of its protein function and anti-adenovirus drugs.

HLA-A胞外区成熟肽基因的克隆及其原核表达载体的构建

根据GenBank基因库中HLA-A胞外区成熟肽基因序列设计2对引物,用RT-PCR法从健康人血液中扩增HLA-A胞外区基因,扩增产物进行T-A克隆、测序.结果表明,获得的HLA-A胞外区基因大小为819bp,与模板序列的同源性为96%.利用基因重组技术,将HLA-A胞外区基因亚克隆入pET-21a(+)载体中.经PCR、酶切和测序鉴定,证实所获重组表达质粒pET–21/HLA-A中含有目的片段,且连接、构建正确,表明成功构建了重组表达质粒pET–21/HLA-A.

Extracellular and cytoplasmic regions of LRIG1 play a negative role in EGFR activity: Findings of a radioligand-binding assay

Objective Leucine-rich repeats and immunoglobulin-like domains 1(LRIG1) is a newly identified human gene that inhibits the epidermal growth factor receptor(EGFR), which on combining with a ligand, can drive tumor growth. This study investigated the interaction between human LRIG1 and EGFR and attempted to delineate the functions of as well as the mechanisms used by the extracellular(ECD) and cytoplasmic(CPD) domains of the human LRIG1 protein to downregulate human EGFR signaling activity.Methods Two constructed chimeric eukaryotic expression vectors, pIRES2-EGFP-3XFLAG-LRIG1-ET and p3FLAG-LRIG1-TC, encoding the extracellular and transmembrane regions(LRIG1-ET) and the transmembrane and cytoplasmic regions(LRIG1-TC), respectively, and the plasmid p3XFLAG-CMV-9-LRIG1 encoding full-length LRIG1(LRIG1-FL) were transfected into the human glioma cell line U251 or primary astrocytoma cells by using liposomes. The number and affinity of cell surface EGFR on transfected cells was determined by ^(125)I-EGF binding assay. Results The dissociation constant(KD) values for EGFR were higher, and the maximum increase was observed in the cells transfected into LRIG1-ET(1.36 folds). The number of maximal binding sites(Bmax) of the receptors was decreased in all transfected cells; the maximum decrease was noted in the cells transfected into LRIG1-FL(40.05%).Conclusion Both the ECD and CPD of LRIG1 are important to negate EGFR signaling. The ECD may interfere with the binding between EGFR and its ligand and facilitate the functions of CPD. The CPD may, when brought in proximity to EGFR, enhance receptor degradation. These two mechanisms can contribute to the downregulation of EGFR-mediated signaling by LRIG1.

非洲猪瘟病毒CD2v蛋白胞内域与胞外域的原核表达及其抗原性分析

【目的】应用大肠杆菌表达系统表达非洲猪瘟病毒(African swine fever virus,ASFV)CD2v蛋白胞外域(N-端,CD2v-N)与胞内域(C-端,CD2v-C)并分析两者的抗原性,为ASFV检测方法的研发提供试验依据和指导。【方法】构建CD2v-N和CD2v-C的重组原核表达质粒,在体外表达并纯化CD2v-N和CD2v-C蛋白,通过Western blotting对表达蛋白进行鉴定;用表达的CD2v-N和CD2v-C蛋白分别肌内接种免疫新西兰大白兔,共免疫3次,每次间隔2周;每次免疫后14 d,应用ELISA方法测定CD2v-N或CD2v-C的特异性抗体水平;用纯化后的CD2V-N和CD2v-C蛋白作为包被抗原,通过ELISA方法检测95份ASFV感染猪的血清CD2v-N或CD2v-C特异性抗体,比较CD2v-N和CD2v-C在猪体内诱导的免疫反应水平。【结果】重组蛋白CD2v-N和CD2v-C分别以包涵体和可溶性形式表达,分子质量分别为22.9和34.0 ku,均能与猪抗ASFV血清特异性结合;用CD2v-N蛋白首免家兔后14 d,血清中未检测到特异性抗体,而在CD2v-C首免的家兔血清中检测到了高滴度的特异性抗体;三免后14 d,CD2v-N和CD2v-C蛋白免疫家兔的血清特异性抗体效价分别为1∶125000和1∶107;ELISA检测结果显示,ASFV感染猪的血清中CD2v-C特异性抗体水平显著高于CD2v-N(P<0.05)。【结论】本研究表达了ASFV CD2v蛋白胞内域和胞外域,前者的抗原性比后者高,CD2v胞内域作为ASFV免疫学检测技术研究与开发的靶标更具优势。该研究结果对ASFV检测方法的研究与开发具有重要指导意义。

中性粒细胞胞外诱捕网通过CCDC25促进骨肉瘤细胞增殖、迁移和侵袭的作用研究

目的探究中性粒细胞胞外捕获网(neutrophil extracellular traps,NETs)在骨肉瘤细胞增殖、迁移和侵袭中的作用及其相关机制。方法纳入骨肉瘤患者和健康受试者各20例,通过ELISA检测血清中PAD4和H3cit水平。提取两组人群外周血中性粒细胞,比较NETs形成差异。将NETs与骨肉瘤细胞MG63共孵育,期间加入DNA降解酶DNaseⅠ,分为对照组、NETs组和NETs+DNaseⅠ组。通过蛋白质印迹检测CCDC25蛋白表达水平,CCK8检测细胞增殖水平,Transwell检测细胞迁移和侵袭水平。将si-NC和si-CCDC25转染至MG63,加入NETs共孵育,分为si-NC组和si-CCDC25组,通过蛋白质印迹检测CCDC25蛋白表达水平,CCK8检测细胞增殖水平,Transwell检测细胞迁移和侵袭水平。结果与健康受试者比较,骨肉瘤患者血清中PAD4和H3cit水平升高(P<0.05),NETs形成能力增强。与对照组比较,NETs组CCDC25蛋白表达升高,细胞增殖、迁移和侵袭水平升高(P<0.05)。与NETs组比较,NETs+DNaseⅠ组CCDC25蛋白表达降低,细胞增殖、迁移和侵袭水平降低(P<0.05)。与si-NC组比较,si-CCDC25组CCDC25蛋白表达降低,细胞增殖、迁移和侵袭水平降低(P<0.05)。结论NETs通过释放的DNA激活骨肉瘤细胞CCDC25表达,从而促进肿瘤细胞增殖、迁移和侵袭。

异钩藤碱对大鼠急性胰腺炎细胞的炎症和凋亡改善及ERK信号通路调控作用

目的观察异钩藤碱(LSO)对大鼠急性胰腺炎(AP)细胞炎症和凋亡改善及ERK信号通路调控作用。方法将AR42J细胞分为6组,对照组正常培养,模型组、LSO组、抑制剂组、LSO+抑制剂组、LSO+激活剂组加入100 nmol/L雨蛙素制备AP细胞模型,LSO组制模后加入40μmol/L LSO,抑制剂组制模后加入10μmol/L U0126,LSO+抑制剂组制模后加入40μmol/L LSO和10μmol/L U0126,LSO+激活剂组制模后加入40μmol/L LSO和0.1μmol/L C16-PAF。采用ELISA法、EdU法及Hoechst 33258染色法分别测定细胞培养液中的炎症因子(TNF-α、IL-6、IL-8、IL-1β)、细胞增殖率和凋亡率,qPCR法测定细胞中NLRP3、斑点样蛋白(ASC)、半胱氨酸蛋白酶-1(Caspase-1)mRNA,WB法测定细胞中ERK 1/2、p-ERK 1/2、NLRP3、ASC、Caspase-1蛋白。结果与对照组比较,模型组细胞TNF-α、IL-6、IL-8、IL-1β、凋亡率、p-ERK 1/2蛋白及NLRP3、ASC、Caspase-1 mRNA和蛋白升高,增殖率降低(P均<0.05);与模型组比较,LSO组、抑制剂组细胞炎症因子(TNF-α、IL-6、IL-8、IL-1β)、凋亡率、p-ERK 1/2蛋白及NLRP3、ASC、Caspase-1 mRNA和蛋白降低,增殖率升高(P均<0.05);与LSO组比较,LSO+抑制剂组中U0126增强了LSO对细胞上述指标趋势的作用,而LSO+激活剂组中C16-PAF则逆转了LSO对细胞上述指标趋势的作用(P均<0.05)。结论LSO对大鼠急性胰腺炎细胞的炎症和凋亡有改善作用,可能通过调控ERK信号通路来实现。

小鼠抗寨卡病毒包膜蛋白胞外区(Eecto)单克隆抗体的制备

目的制备小鼠抗寨卡病毒(ZIKV)包膜蛋白胞外区(Eecto)单克隆抗体。方法首先构建ZIKV Eecto的原核表达质粒pET28a-ZIKV-Eecto,将其转化至大肠杆菌感受态BL21后,利用异丙基β-D-硫代半乳糖苷(IPTG)诱导表达。重组Eecto蛋白以包涵体形式表达,经过变性、复性和超滤获得纯化的蛋白。将Eecto蛋白3次免疫后,获得多克隆抗体血清,进行效价测定,并利用ZIKV prME真核表达质粒转染的HEK293T细胞进行Western blot法和免疫荧光法分析。取效价较高的小鼠脾脏制备脾细胞,与SP2/0骨髓瘤细胞融合,通过有限稀释法获取分泌抗体的杂交瘤细胞,并进一步制备腹水。对腹水进行抗体效价测定、亚类分析。以ZIKV同属病毒日本脑炎病毒(JEV)、黄热病病毒(YFV)、登革病毒1-4(DENV1-4)、蜱传脑炎病毒(TBEV)的Eecto为包被抗原,利用ELISA分析ZIKV单克隆抗体的交叉反应性,进一步对效价高、特异性强的抗体进行特异性分析。结果成功构建了原核表达质粒pET28a-ZIKV-Eecto,并获得纯化的Eecto蛋白,该蛋白具有良好的免疫原性;制备筛选得到1D6、4F11、4H7、4F8四株单克隆抗体,其中三株(1D6、4H7、4F8)为IgGκ型抗体,一株(4F11)为IgMκ,1D6腹水效价大于1∶108;其中1D6和4H7为ZIKV特异性抗体,与其他黄病毒无交叉反应。结论成功制备了小鼠抗ZIKV Eecto单克隆抗体,为后续建立ZIKV检测方法及致病机制研究提供了实验材料。

脓毒症患者血清NLRC3、ECM1表达与急性呼吸窘迫综合征的相关性研究

目的探讨脓毒症患者血清NOD样受体家族含CARD结构域蛋白3(NLRC3)、细胞外基质蛋白1(ECM1)表达与急性呼吸窘迫综合征(ARDS)的相关性。方法选取脓毒症患者133例纳入脓毒症组,并选取同时间段体检健康者80例纳入对照组。根据是否并发ARDS分为ARDS组(52例)和非ARDS组(81例),采用酶联免疫吸附法检测血清NLRC3、ECM1表达。通过多因素Logistic回归分析筛选脓毒症患者并发ARDS的因素。采用受试者工作特征(ROC)曲线分析血清NLRC3、ECM1表达对脓毒症患者并发ARDS的预测价值。结果与对照组比较,脓毒症组血清NLRC3表达降低,ECM1表达升高,差异有统计学意义(P<0.05)。133例脓毒症患者ARDS发生率为39.10%(52/133)。与非ARDS组比较,ARDS组血清NLRC3表达降低,ECM1表达升高,差异有统计学意义(P<0.05)。脓毒症患者并发ARDS的独立危险因素为序贯器官衰竭评估评分增加、血乳酸升高、ECM1升高,独立保护因素为NLRC3升高(P<0.05)。血清NLRC3、ECM1表达联合预测脓毒症患者并发ARDS的曲线下面积为0.887,大于血清NLRC3、ECM1表达单独预测的0.811、0.792(P<0.05)。结论脓毒症患者血清NLRC3表达降低和ECM1表达升高与并发ARDS密切相关。血清NLRC3、ECM1表达联用对脓毒症患者并发ARDS有较高的预测价值。

黄芪多糖在Her-2阳性乳腺癌患者化疗中增效减毒的作用及其对血清Her-2-ECD、TAP和疗效的影响

目的:探讨黄芪多糖在人表皮生长因子受体-2(human epidermal growth factor receptor-2,Her-2)阳性乳腺癌患者化疗中增效减毒的作用及其对血清人表皮生长因子受体-2胞外段(human epidermal growth factor receptor-2-extracellular domain,Her-2-ECD)、肿瘤异常糖链糖蛋白(tumor abnormal protein,TAP)和疗效的影响。方法:选择2020年1月—2023年6月新余北湖医院收治的90例Her-2阳性乳腺癌患者作为研究对象,将患者随机分为对照组和观察组,各45例。两组均给予TCbHP(多西他赛+卡铂+曲妥珠单抗+帕妥珠单抗)方案治疗;观察组在此基础上给予注射用黄芪多糖治疗。比较两组治疗前后的中医症候积分、血清Her-2-ECD、TAP水平、免疫功能(CD4^(+)、CD8^(+))、白细胞(white blood cell,WBC)水平、乳腺癌患者的生活质量量表(functional assessment of cancer therapy-breast,FACT-B)评分、疗效及不良反应发生率。结果:治疗前,两组各项中医症候积分、Her-2-ECD、TAP、CD4^(+)、CD8^(+)、WBC、FACT-B评分比较,差异均无统计学意义(P>0.05)。治疗后,观察组各项中医症候评分、Her-2-ECD、TAP、CD8^(+)、FACT-B各项评分及不良反应发生率均低于对照组,CD4^(+)、WBC、总有效率均高于对照组,差异均有统计学意义(P<0.05)。结论:黄芪多糖能够改善Her-2阳性乳腺癌化疗患者的化疗效果,减轻化疗带来的毒性反应,提高患者的生活质量。

狂犬病病毒糖蛋白膜外区基因在大肠埃希氏菌中的高效表达

为获得狂犬病病毒(RV)糖蛋白抗原,采用RT-PCR方法从狂犬病病毒ERA株中扩增了编码RV糖蛋白的全长基因,将其克隆于pMD18-T载体,再经PCR扩增出糖蛋白全长基因和膜外区基因,将其分别亚克隆至原核表达载体pET-28a(+)、pET-32a(+)和pGEX-4T-1中,经PCR 和双酶切鉴定以及序列分析,表明已成功构建了重组质粒。将重组质粒转化到大肠埃希氏菌BL21 (DE3)中进行表达,结果显示,克隆到pET-32a(+)的糖蛋白膜外区基因表达量最高,目的蛋白表达量占菌体总蛋白的45．4％。经Western-blotting检测,不同载体表达的糖蛋白膜外区产物均可与兔抗RV多抗发生特异性反应,表明,重组蛋白具有良好的反应原性。

抗人晚期糖基化终产物受体胞外段不同表位单克隆抗体的制备

目的 制备抗人晚期糖基化终产物受体(RAGE)胞外段单克隆抗体。方法 用纯化人重组RAGE胞外段(氨基酸序列23～342)免疫Balb／c小鼠，取其脾细胞与NS—1融合制备杂交瘤，经筛选和两次克隆化，从制备的腹水中纯化单克隆抗体。结果和结论 获得两株杂交瘤细胞B2．2和E10，其分泌单抗的亚型均为IgG2b。经ELISA、Westernblot和流式细胞仪鉴定，证明两株单抗均可结合重组RAGE及表达于细胞表面的RAGE，且两株抗体识别的位点为远隔表位，所建立的双夹心法可用于检测可溶性重组RAGE。这两株抗体将为研究RAGE相关疾病提供有效的工具。

人Toll-like receptor 2胞外段的克隆和表达

目的 克隆、表达人Toll-like receptor2(TLR2)胞外段(A26-T588)基因,获得人TLR2胞外段蛋白。方法 RT-PCR扩增TLR2胞外段基因,以pcDNA3.1+质粒为载体在HEK293细胞中表达TLR2胞外段蛋白,同时以pcDNA3.1+/TLR2(A26-T588)重组质粒免疫昆明鼠,制备抗TLR2胞外段蛋白多抗。结果 PCR扩增及重组质粒测序结果表明成功地构建了pcDNA3.1+/TLR2(A26-T588)真核表达质粒,SDS-PAGE分析纯化产物在M_r为68000处出现明显蛋白条带。重组质粒DNA免疫小鼠3次后,血清抗体滴度可达1∶250。TLR2胞外段蛋白可与LPS结合,并在一定的质量浓度范围内呈剂量依赖性。结论 构建的pcDNA3.1+/TLR2(A26-T588)真核表达质粒可在哺乳动物细胞中表达TLR2胞外段蛋白,并与重组质粒DNA免疫小鼠抗血清及TLR2单克隆抗体TL2.1特异性反应,由此证明其表达正确。

肝癌相关抗原HAb18G胞外区片段的原核表达与免疫学活性分析

目的 :利用大肠杆菌高效表达肝癌相关抗原HAb18G胞外区片段 ,并分析其与相应抗体的结合活性 ,进而明确表达产物用于筛选基因工程抗体的可行性 .方法 :用PCR技术扩增出HAb18G胞外区基因片段 ,克隆入原核表达载体pGEX 4T 3中 ,筛选及鉴定阳性重组子 ,IPTGv诱导表达后对表达产物进行纯化及复性等处理 ,同时利用SDS PAGE ,Western Blot以及ELISA等方法检测蛋白表达情况及其免疫学特性 .结果 :成功构建了肝癌相关抗原HAb18G胞外区片段的原核表达载体 pGEX 4T 3/HAb18GE ,并在大肠杆菌中成功实现高效融合表达 .表达蛋白Mr 4 6 0 0 0 ,表达量约占菌体总蛋白量的 4 3% ,表达产物主要以包涵体形式为主 .另外 ,表达蛋白在变性和非变性的条件下均可以与HAb18GmAb特异性结合 .结论 :原核融合表达的HAb18G胞外区片段可以替代天然的HAb18G蛋白 ,以用做抗原来筛选新型的基因工程抗体 .

人DC-SIGN全长编码区基因的克隆及其胞外段的原核表达

目的:克隆人DC-SIGN全长编码区基因,获得其胞外段的原核表达产物。方法:采用RT-PCR方法,从健康产妇胎盘中克隆DC-SIGN全长cDNA,扩增其胞外段基因并构建pET41a-sDC-SIGN重组表达质粒,在大肠杆菌BL21(DE3)中表达,以SDS-PAGE和Western blot鉴定表达产物。结果:从健康产妇胎盘总RNA中,扩增获得约1300bp的DNA片段,克隆至pGM-T载体获得重组质粒pGM-DC-SIGN。从pGM-DC-SIGN扩增DC-SIGN的胞外段基因,构建重组表达质粒pET-41a-sDC-SIGN;纯化表达产物sDC-SIGN-GST,鉴定其相对分子质量(Mr)为66000,Western blot证明其可与抗DC-SIGN抗体特异性结合。结论:成功克隆DC-SIGN全长编码区基因,并在大肠杆菌中成功表达其胞外段融合蛋白sDC-SIGN-GST,为进一步研究DC-SIGN的功能奠定了基础。

CTLA4胞外区蛋白在GS115酵母中的表达和活性鉴定

目的 获取具有生物学活性的CTLA4胞外区蛋白。方法 构建CTLA4胞外区 (CTLA412 5)蛋白的酵母表达载体 ,在GS115酵母细胞中表达。通过硫酸铵粗分离和离子交换层析等 ,获取纯化的目的蛋白 ,并在CTLL2细胞中鉴定活性。结果 质粒在GS115酵母中可较高水平地表达CTLA4胞外区蛋白。经纯化后的蛋白可抑制IL 2刺激的CTLL2细胞的增殖。结论 GS115酵母可高效表达具有生物学活性的CTLA4胞外区蛋白。

1人TLR4胞外区基因重组腺病毒载体的构建与鉴定

目的构建并鉴定人TLR4胞外区基因重组腺病毒载体。方法以pUCm-TLR4质粒为模板,运用PCR技术扩增TLR4胞外区目的基因片段,片段回收后经酶切连接穿梭质粒pAdTrack-CMV上,获得重组腺病毒质粒pAdTrack-CMV-TLR4.通过KpnⅠ和HindⅢ双酶切,测序鉴定后,将鉴定正确的质粒经PmeI酶切线性化后,转化到含有腺病毒骨架质粒pAdEasy-1的感受态细菌BJ5183中,进行同源重组,卡那抗性筛选阳性克隆,提取质粒,用脂质体介导转染293细胞,通过观察绿色荧光蛋白(GFP)的表达及PCR技术,Western blot等方法鉴定重组腺病毒,并进行病毒滴度测定。结果人TLR4胞外区基因重组腺病毒载体构建正确,病毒滴度为3.2×109pfu/mL。结论成功构建了人TLR4胞外区基因重组腺病毒载体,为下一步实验奠定基础。

狂犬病病毒糖蛋白胞外区基因的原核表达、纯化及鉴定

利用RT-PCR技术,将狂犬病病毒株ERA株糖蛋白胞外区基因分两段进行扩增,经克隆与序列分析,两片段大小分别为523,381 bp,各编码174,127个氨基酸,分子量分别为19.7,14.5 kDa。在原核表达载体pET-43a中分别克隆了这两段糖蛋白基因,将重组质粒转化到表达菌BL21(DE3)中,经SDS-PAGE电泳分析,在分子量约为94,89kDa处分别出现新蛋白带,和预期的目的蛋白的分子量相符。两重组蛋白主要以可溶形式表达,利用Ni2+亲和层析柱纯化了蛋白,纯度大于95%。Western-Blot分析结果显示,两种重组融合蛋白均可与兔抗RBV多抗血清反应,具有良好的反应原性。

proBDNF对培养的海马神经元存活的影响及其机制

目的:初步探讨proBDNF(precursor of brain-derived neurotrophic factor)对海马神经元的可能作用及其机制。方法:采用体外培养胚鼠海马神经元,并给予proBDNF,preBDNF(propeptide of proBDNF)和抗proBDNF血清处理;30min,1h和48h后行尼氏染色,ELK-p(Ets domain protein),ErK2(extracellularsignal regulated kinase)和c-fos免疫细胞化学染色。结果:给予proBDNF处理后,可见培养细胞内ELK-p,ErK2和c-fos表达明显上调,部分细胞核深染;而用抗血清中和内源性proBDNF后,ELK-p、ErK2和c-fos均下调,且细胞出现肿胀、空泡样变化。preBDNF处理组细胞与正常对照组类似。结论:proBDNF可维持海马神经元的存活,其机制可能与激活ErK和ELK信号通路有关。