Construction and Identification of Mammary Gland-specific Expression Vector of Bovine Tracheal Antimicrobial Peptide (TAP)

[ Objective] This study aimed to construct nmnmm_ry gland-specific expression vector of bovine tracheal antimicrobial peptide （TAP） gene. [ Method] TAP gene of dairy cattle was amplified from the mammary gland tissue by RT-PCR using a pair of primers which were designed according to bovine TAP cDNA se- quence （NM_174776） in GenBank, and then cloned into pMD19-T Simple vector for sequencing. The recombinant plasmid was digested using EcoRI and KpnI, the target gene fragment was recovered and inserted into general mammary gland-specific expression vector pBLG-EGFP harboring enhanced green fluorescent protein （ EGFP）, and transfected into bovine mammary epithelial cells （bMEC）, COS-7 cells and lactating rabbit mmmnary gland tissue by lipofectin transfection. The ex- pression of green fluorescent protein in transfected cells was detected under fluorescence microscopy, and the expression of TAP mRNA in rabbit mammary gland tis- sue was detected by semi-quantity RT-PCR. [ Result] The constructed mammary gland-specific expression vector pBLG-EGFP-TAP specifically expressed EGFP in transfected bMECs. In addition, semi-quantitative RT-PCR result showed that the expression level of TAP mRNA in rabbit mammary gland tissue was significantly enhanced after transfeeted with pBLG-EGFP-TAP. [ Conclusion] The mammary gland-specific expression vector pBLG-EGFP-TAP was successfully constructed, which provided important materials for further investigation of expression characteristics of TAP gene and prevention of bovine mastitis by using genetic engineering technology.

奶牛乳房炎抗性基因TAP cDNA克隆及序列分析

采用RT-PCR方法从奶牛乳腺组织中扩增气管抗菌肽(TAP)基因,重组到pMD19-T Simple载体中,并进行序列分析。序列分析结果显示,克隆的TAP基因包含完整的开放阅读框(ORF)195 bp,与牛TAP基因同源性达93.8%;该ORF编码的64个氨基酸,含有β-防御素特征性结构即6个在特定位置上的保守半胱氨酸残基。TAP基因cDNA完整开放阅读框的克隆,为进一步开发应用重组牛β-防御素奠定了基础。

针刺公孙、四缝穴配合脏腑点穴对胃肠结热型小儿肠系膜淋巴结炎的疗效观察

目的分析针刺公孙、四缝穴配合脏腑点穴对小儿肠系膜淋巴结炎(胃肠结热型)的疗效以及对血清肠型脂肪酸结合蛋白(I-FABP)、血管活性肠肽(VIP)的影响。方法选择肠系膜淋巴结炎(胃肠结热型)患儿60例为研究对象,根据随机数字表法分为对照组(n=30,予常规治疗+针刺公孙、四缝穴)与研究组(n=30,在对照组基础上配合使用脏腑点穴)。比较2组临床疗效、主要症状与体征变化,并检测血清I-FABP、VIP表达水平。结果研究组治疗总有效率高于对照组,差异有统计学意义(P<0.05)。治疗2周后,2组血清I-FABP水平较治疗前降低,且研究组血清I-FABP水平低于对照组,差异有统计学意义(P<0.05);治疗2周后,2组血清VIP水平较治疗前升高,且研究组血清VIP水平高于对照组,差异有统计学意义(P<0.05)。治疗2周后,研究组主要症状与体征改善程度优于对照组,差异有统计学意义(P<0.05)。结论针刺公孙、四缝穴配合脏腑点穴可用于治疗胃肠结热型小儿肠系膜淋巴结炎,能够调理和改善胃肠道功能,调节血清I-FABP、VI水平,缓解患儿主要症状与体征,临床可作为一种有效的治疗方法。

奶牛气管抗菌肽(TAP)基因乳腺特异性表达载体的构建与鉴定

【目的】构建奶牛气管抗菌肽(TAP)基因乳腺特异性表达载体。【方法】根据GenBank中牛TAP基因cDNA序列(GenBank号:NM_174776)设计引物,从奶牛乳腺组织中RT-PCR扩增TAP基因编码序列,将其克隆到pMD19-T(simple)载体中测序。重组质粒pMD-TAP经EcoRⅠ+KpnⅠ双酶切回收目的基因片段,亚克隆到携带增强型绿色荧光蛋白的通用型乳腺特异性表达载体pBLG-EGFP中,采用脂质体法转染奶牛乳腺上皮细胞(bMEC)、COS-7细胞,并注射泌乳家兔乳腺组织,荧光显微镜检测转染细胞中绿色荧光蛋白的表达,半定量RT-PCR检测家兔乳腺组织中TAP mRNA的表达。【结果】成功构建了乳腺特异性表达载体pBLG-EGFP-TAP,该载体可在bMEC中特异性地表达绿色荧光蛋白;半定量RT-PCR检测发现,转染pBLG-EGFP-TAP可显著提高家兔乳腺组织中TAPmRNA的表达水平。【结论】成功构建了乳腺特异性表达载体pBLG-EGFP-TAP,为进一步研究奶牛TAP基因的表达特性及利用基因工程技术防治奶牛乳房炎提供了重要材料。

肝癌H-22细胞膜抗原肽提取物对小鼠免疫功能的影响及其抑瘤作用

目的 应用小鼠肝癌H 2 2细胞膜相关抗原肽 (TAP)提取物免疫小鼠 ,观察其对小鼠自身移植肿瘤生长及免疫学参数的影响 ,为制备肿瘤疫苗提供实验依据。方法 采用微酸洗脱法制备分子量≤ 30 0 0Da的细胞膜TAP提取物 ,皮下免疫小鼠 ,检测胸腺细胞增殖反应、T细胞亚组百分数的变化 ,脾细胞ConA反应性、IL 2和IFN γ活性、CTL杀伤活性的变化及抑瘤效应。结果 TAP提取物免疫后 ,移植肿瘤的发生率降低 (P <0 .0 1) ,平均出现时间延迟 (P <0 .0 0 1) ,生长速度减慢 ;同时 ,脾细胞ConA反应性 (P <0 .0 1)、IFN γ(P <0 .0 5 )和IL 2分泌活性和CTL杀伤活性 (P <0 .0 5 )不同程度增强 ;胸腺细胞3 H TdR自发掺入率 (P <0 .0 5 )及CD4 + 和CD8+ T细胞百分数 (P <0 .0 5 )也有不同程度增高。结论 小鼠肝癌H 2 2细胞膜TAP提取物具有免疫原性 ,能有效激发免疫系统功能 ,抑制自身移植肿瘤的生长。

新型多肽表位技术研究进展

多肽表位作为抗原的重要组成成分,可以被宿主免疫系统B细胞产生的抗体(Ig)和T细胞受体(TCR)识别,从而诱导机体产生免疫保护作用。传统的研究方法如交叠肽合成等费时费力,极大地限制了多肽表位的研究。随着生物信息学、高通量测序、CRISPR/Cas9、质谱(MS)等技术出现以及TAP非依赖型蛋白加工机制的不断阐述,使表位的研究得到不断完善。作者介绍了最新的多肽表位研究方法,包括利用计算机对B细胞和T细胞表位的预测、基于MHC与抗原肽结构作用为基础的方法、结合高通量测序技术的表位筛选方法、结合新型基因编辑技术的表位筛选方法、TAP非依赖性T细胞表位的最新研究等,并对今后多肽表位研究的发展进行了展望。

嵌合KGDS基序的蜱抗凝血肽突变体基因在大肠埃希菌BL21(DE3)中的表达

目的设计含赖氨酸-甘氨酸-天冬氨酸-丝氨酸基序(KGDS)的蜱抗凝血肽(TAP)突变体基因序列,并在大肠埃希菌BL21(DE3)中与硫氧还蛋白(Trx)融合表达,以获得Trx-TAP-KGDS融合蛋白。方法人工合成目的基因,定向克隆于含Trx基因的高效原核表达载体pET32a(+),构建重组质粒pET32a(+)-TAP-KGDS,并转化BL21感受态菌,以PCR及双酶切鉴定阳性克隆;含正确重组质粒的工程菌经IPTG诱导表达,SDS-PAGE电泳鉴定表达产物。结果重组质粒经PCR及双酶切鉴定,均获得约209 bp的基因片段,与预期大小一致;SDS-PAGE分析显示,含重组质粒的工程菌在IPTG的诱导下高效表达分子质量单位约为24 ku的蛋白质,该蛋白以水溶性形式为主。结论构建了含KGDS基序的TAP突变基因的原核表达载体pET32a(+)-TAP-KGDS,并成功进行了融合表达,为进一步研究其抗凝血活性打下了基础。

Investigation on the effect of peptides mixture from tumor cells inducing anti-tumor specific immune response

The peptides mixture was prepared from tumor cells by freezing-thawing cells, precipitation by heating, followed by acidification of the solution. The activation and proliferation of mouse splenocytes by HSP70-peptide complex, formed by the binding of HSP70 and peptides in vitro, were observed, so was the specific cytotoxicity of the proliferative lymphocytes to tumor cells. The phenotypes of the proliferative lymphocytes were analyzed by a flow cytometer. BALB/c mice inoculated with H22 hepatocarcinoma cells in peritoneal cavity or hind thigh were immunized by injection with HSP70-peptides complex to observe the inhibitory effect of the immunization on tumor and lifetime of tumor-bearing mice. On the other hand, blood samples were collected from the immunized mice to check the functions of liver and kidney. The results showed that the peptides mixture from tumor cells contained tumor-specific antigen peptides which could be presented by HSP70 to activate lymphocytes in vitro, the proliferative lymphocytes were T cells which were specifically cytotoxic to tumor cells, the in vivo growth of both ascitic and solid carcinoma could be suppressed by immunization with HSP70-peptides and the lifetime of tumor-bearing mice was prolonged, the in vivo immunization with HSP70-H22-peptides had no impact on the function of mouse liver and kidney, suggesting that there was no occurrence of autoimmunity in vivo after immunization.

Advances in Structure-function Relationships and Mechanism of Transporter Associated with Antigen Processing

The transporter associated with antigen processing （TAP） belongs to the ATP-binding cassette （ABC） transporter superfamily. Driven by ATP hydrolysis, TAP translocates antigenic peptides from the cytosol into the ER （endoplasmic reticulum） lumen where the antigenic peptides are loaded onto the HLA class I molecules. Recently, numerous studies show that TAP is closely related with various diseases such as viral infections, autoimmune diseases, and different malignancies. In consideration of important roles of TAP in human adaptive immunity, this review summarizes the recent advances in structure-function relationships of crucial domains and transport mechanism systematically. The challenging problems and potential methods are also pointed out for in-depth researches.

抗炎抗凝双效融合蛋白TAP-SSL5的药理学分析

目的分析抗炎抗凝双效融合蛋白TAP-SSL5对动物的药理作用,为其安全性用药提供实验依据。方法取昆明(KM)小鼠,经尾静脉分别注射1、3和9 mg/kg TAP-SSL5,观察其对小鼠神经系统的影响;取SD大鼠,经尾静脉分别注射1和3 mg/kg TAP-SSL5,设溶剂[20 mmol/L甘氨酸(Gly)-NaOH缓冲液,pH 10.6]为对照组,观察其对呼吸系统和心血管系统的影响。结果 TAP-SSL5对KM小鼠一般行为状态、协调机能和戊巴比妥钠阈下剂量催眠的协同作用无明显影响;对SD大鼠的血压、呼吸频率和心率无明显影响,与溶剂对照组比较,差异无统计学意义(P均>0.05)。结论融合蛋白TAP-SSL5对动物的神经系统、呼吸系统和心血管系统无明显影响,表明其具有较好的安全性,且无明显的毒副作用。

EB病毒蛋白BNLF2a阻止抗原转运蛋白TAP的构象变化

【背景】EB病毒是一个常见的病原,它能引起霍奇金淋巴瘤、伯基特淋巴瘤以及胃癌、鼻咽癌。该病毒编码的膜蛋白BNLF2a抑制抗原转运蛋白TAP (Transporter associated with antigen processing)从而逃逸T细胞的清除。TAP属于ABC(ATP-bindingcassette)转运蛋白超家族,是由TAP1和TAP2两个亚基构成的。TAP通过ATP提供能量,跨膜转运抗原多肽,这一过程伴随着构象变化。【目的】旨在揭示BNLF2a是否影响TAP的构象变化。【方法】TAP蛋白核酸结合结构域的二聚体界面的D-loop进行点突变,引入半胱氨酸。在表达和不表达BNLF2a情况下,采用氧化性的二价铜离子交联半胱氨酸,并通过Westernblot对比TAP的半胱氨酸形成二硫键的比例。【结果】BNLF2a表达使TAP被交联的比例增高。【结论】BNLF2a可能将TAP稳定在核苷酸结合结构域二聚化的构象,从而同时抑制ATP和抗原多肽结合到TAP上来。

肿瘤相关抗原肽与低剂量全身照射的协同抑瘤作用

目的观察低剂量X射线照射对小鼠肝癌H-22细胞膜相关抗原肽(TAP)提取物的抑瘤作用及免疫学功能的影响,为低剂量辐射(LDR)与肿瘤疫苗联合治疗肿瘤提供实验依据。方法采用微酸洗脱法制备相对分子质量≤3×106的细胞膜TAP提取物,先给予小鼠75mGyX射线全身照射,12h后以TAP提取物皮下免疫小鼠,检测脾细胞CD3、CD69和TCRαβ表面标记、脾T细胞亚组百分数的变化、脾细胞ConA反应性、IL-2和IFN-γ活性、CTL杀伤活性的变化及抑瘤效应。结果小鼠经TAP提取物免疫后,移植肿瘤的发生率降低,肿瘤平均出现时间延迟,生长速度减慢;脾细胞CD3分子和CD69分子的表达显著升高,脾细胞ConA反应性、IFNγ分泌活性和CTL杀伤活性显著增强,IL-2分泌增多。而同时给予LDR的小鼠不仅上述功能不同程度增强,脾CD8+细胞百分数显著增高。结论LDR与细胞膜TAP具有协同抑瘤作用,细胞免疫力的明显增强可能为其机制之一。