Construction, Expression and Identification of a Recombinant BCG Vaccine Encoding Human Mycobacterium Tuberculosis Heat Shock Protein 65

Heat shock protein 65 (HSP65) is one of the most important protective immunogens against the tuberculosis infection. The signal sequence of antigen 85B and the whole HSP65 DNA sequence of human Mycobacterium tuberculosis (M. tuberculosis) were amplified from BCG genome and plasmid pCMV-MTHSP65 respectively by polymerase chain reactions (PCR). These two sequences were cloned into the plasmid pBCG-2100 under the control of the promoter of heat shock protein 70 (HSP70) from human M. tuberculosis, yielding the prokaryotic shuttle expression plasmid pBCG-SP-HSP65. Results of restriction endonuclease analysis, PCR detection and DNA sequencing analysis showed that the two cloned DNA sequences were consistent with those previously reported, and the direction of their inserting into the recombinant was correct and the reading frame had been maintained. The recombinants were electroporated into BCG to construct the recombinant BCG vaccine and induced by heating. The induced expression detected by SDS-PAGE showed that the content of 65 kD protein expressed in recombinant BCG was 35.69 % in total bacterial protein and 74.09 % in the cell lysate supernatants, suggesting that the recombinant HSP65 gene could express in BCG with high efficiency and the expressed proteins were mainly soluble. Western-blot showed that the secretive recombinant proteins could specifically combine with antibody against M. tuberculosis HSP65, indicating that the recombinant proteins possess the biological activity of HSP65.

Recent advances in heat shock protein-based cancer vaccines

BACKGROUND: Active immunotherapy has been successful in preventing many infectious diseases, and is being explored for its anti-tumor use. Purified antigens, peptides, gene-based systems and antigens contained in whole cells or cell lysates are used in specific active immunotherapy for cancer, known as cancer vaccines. Cancer vaccines do not directly kill tumor cells, but prime a specific humoral and/or cellular immune response against the tumor. Up to date, many kinds of cancer vaccines have been tested in the world and have shown their own advantages. Heat shock protein (HSP)-based cancer vaccine is one of the outstanding representatives. In this paper, we review recent advances in HSP-based cancer vaccines. DATA SOURCES: An English-language literature search was conducted using MEDLINE (1990-2005) on HSP, cancer vaccines and other related subjects. RESULTS: Several kinds of HSP-based cancer vaccines which have been explored worldwide, include tumor derived HSP-pepdde complex cancer vaccines, artificially reconstituted HSP-peptide complex cancer vaccines, HSPpeptide fusion protein cancer vaccines and HSP-based DNA cancer vaccines, etc. Many HSP-based cancer vaccines are being tested in clinical trials, and some are being tested in phase Ⅲ clinical trials at present. CONCLUSION: The available results in preclinical tests and clinical trials indicate that HSP-based cancer vaccines are promising in cancer therapy.

Targeting hepatitis B virus antigens to dendritic cells by heat shock protein to improve DNA vaccine potency

AIM： To investigate a novel DNA vaccination based upon expression of the HBV e antigen fused to a heat shock protein （HSP） as a strategy to enhance DNA vaccine potency.METHODS： A pCMV-HBeAg-HSP DNA vaccine and a control DNA vaccine were generated. Mice were immunized with these different construct. Immune responses were measured 2 wk after a second immunization by a T cell response assay, CTL cytotoxicity assay, and an antibody assay in C57BL/6 and BALB/c mice. CT26-HBeAg tumor cell challenge test in vivo was Performed in BALB/c mice to monitor anti-tumor immune responses.RESULTS： In the mice immunized with pCMV-HBe-HSP DNA, superior CTL activity to target HBV-positive target cells was observed in comparison with mice immunized with pCMV-HBeAg （44% ± 5% vs 30% ± 6% in E： T 〉 50：1, P 〈 0,05）, ELISPOT assays showed a stronger T-cell response from mice immunized with pCMV-HBe- HSP than that from pCMV-HBeAg immunized animals when stimulated either with MHC class I or class Ⅱ epitopes derived from HBeAg （74% ± 9% vs 31% ± 6%, P 〈 0.01）. ELISA assays revealed an enhanced HBeAg antibody response from mice immunized with pCMV- HBe-HSP than from those immunized with pCMV-HBeAg. The lowest tumor incidence and the slowest tumor growth were observed in mice immunized with pCMV- HBe-HSP when challenged with CT26-HBeAg.CONCLUSION： The results of this study demonstrate a broad enhancement of antigen-specific CD4^＋ helper,CD8^＋ cytotoxic T-cell, and B-cell responses by a novel DNA vaccination strategy. They also proved a stronger antigen-specific immune memory, which may be superior to currently described HBV DNA vaccination strategies for the treatment of chronic HBV infection.

The Heat Shock Protein Story—From Taking mTORC1,2 and Heat Shock Protein Inhibitors as Therapeutic Measures for Treating Cancers to Development of Cancer Vaccines

Heat shock proteins (HSPs) serve to correct proteins’ conformation, send the damaged proteins for degradation (quality control function). Heat shock factors (HSFs) are their transcription factors. The protein complexes mTOR1 and 2 (with the same core mTOR), the phosphoinositide-dependent protein kinase-1 (PDK1), the seine/threonine-specific protein kinase (Akt), HSF1, plus their associated proteins form a network participating in protein synthesis, bio-energy generation, signaling for apoptosis with the help of HSPs. A cancer cell synthesizes proteins at fast rate and needs more HSPs to work on quality control. Shutting down this network would lead to cell death. Thus inhibitors of mTOR (mTORI) and inhibitors of HSPs (HSPI) could drive cancer cell to apoptosis—a “passive approach”. On the other hand, HSPs form complexes with polypeptides characteristic of the cancer cells;on excretion from the cell, they becomes antigens for the immunity cells, eventually leading to maturation of the cytotoxic T cells, forming the basic principle of preparing cancer-specific, person-specific vaccine. Recent finding shows that HSP70 can penetrate cancer cell and expel its analog to extracellular region, giving the hope to prepare a non-person-specific vaccine covering a variety of cancers. Activation of anti-cancer immunity is the “active approach”. On the other hand, mild hyperthermia, with increase of intracellular HSPs, has been found to activate the immunity response, and demonstrate anti-cancer effects. There are certain “mysteries” behind the mechanisms of the active and passive approaches. We analyze the mechanisms involved and provide explanations to some mysteries. We also suggest future research to improve our understanding of these two approaches, in which HSPs play many roles.

Enhancement of humoral immune responses to HBsAg by heat shock protein gp96 and its N-terminal fragment in mice

AIM: Most studies on the immune effect of gp96 were focused on its enhancement of CTLs. It is interesting to know whether gp96 could influence the humoral immune response, and whether the recombinant N-terminal fragment of gp96 could substitute native gp96 to stimulate the immune system.METHODS: gp96 isolated from livers of normal mice and its N-terminal fragment (amino acid 22-355) expressed in E coli were used for immunization of BALb/c mice. Eight groups of mice received one of the following regiments subcutaneously in 100 μL phosphate buffered saline (PBS)at an interval of 3 wk. Group 1: PBS only; group 2:gp96 only; group 3: N-terminal fragment only; group 4: HBsAg only; group 5: HBsAg+gp96; group 6: HBsAg+N-terminalfragment; group 7: HBsAg+incomplete Freud's adjuvant; group 8: HBsAg+N-terminal fragment (95 ℃ heated for 30 min). Serum anti-HBsAg antibody levels were assayed by ELISA. CTL responses in splenocytes were analyzed by ELISPOT after the last vaccination.RESULTS: The average titer of serum anti-HBsAg antibodyin the mice immunized with HBsAg together with gp96 or its N-terminal fragment were much higher than those immunized with HBsAg alone detected by ELISA. The cellular immune response of the mice immunized with HBsAg together with gp96 or its N-terminal fragment was not different with those immunized with HBsAg alone measured by ELISPOT assay.CONCLUSION: gp96 or its N-terminal fragment greatly improved humoral immune response induced by HBsAg, but failed to enhance the CTL response, which demonstrated the potential of using gp96 or its N-terminal fragment as a possible adjuvant to augment humoral immune response against HBV infection.

Heat shock protein 72 normothermic ischemia,and the impact of congested portal blood reperfusion on rat liver

INTRODUCTIONFrom the technical aspect of liver surgery ,control of bleeding during hepatic parenchymal resection is one of the most important procedures in hepatectomy .Pringle,s maneuver ,a temporary cross-clamping of the hepatoduodnal ligament ,has often been used for this purpose[1],This is the simplest and userul technique to reduce intraoperative blood loss .

HEAT SHOCK PROTEIN gp96 AND CANCER IMMUNOTHERAPY

Heat shock protein gp96 is a highly conserved and monomorphic glycoprotein in the endoplasmic reticulum.It functions as molecular chaperone and can associate with a variety of antigenic peptides noncovalently in vivo and in vitro. Recent studies have indicated that gp96 molecules participate in major histocompatibility complex class I - restricted antigen presentation pathway. Immunization of mice with gp96 preparations isolated from cancer cells can elicit a cancer - specific protective T cell immune response that is recallable, which is a prerequisite for gp96 as a therapeutic vaccine against cancers. The immunogenicity of gp96 molecules has been attributed to the antigenic peptides associated with them. These phenomena provide a new pathway for cancer immunotherapy. The mechanism that the gp96 -peptide complex induces specific immune response and the explorations for gp96 - peptide complex as a therapeutic cancer vaccine are reviewed.

BCG HSP65-人HER-2/neuT细胞表位融合蛋白基因的扩增及序列分析

目的 :获得卡介苗热休克蛋白 6 5 (BCGHSP6 5 )与人HER 2 /neuT细胞表位 (GP2 )构成的融合蛋白 (BCGHSP6 5 GP2 )基因 ,并对其进行测序。方法 :从卡介苗结核杆菌中提取其基因组DNA ,设计一对寡核苷酸引物 ,采用聚合酶链反应 (PCR)获得BCGHSP6 5基因 ,再设计一对寡核苷酸引物 ,再次PCR ,获得BCGHSP6 5 GP2 基因 ,DNA序列分析BCGHSP6 5 GP2 基因。结果 :本实验采用两轮PCR方法获得的基因片段长度为 170 0bp ,DNA序列分析确证为编码BCGHSP6 5 GP2 融合蛋白的序列。结论 :采用PCR获得BCGHSP6 5 GP2 基因序列是正确的 。

BCG 65KD热休克蛋白的纯化

目的：研究卡介苗（ＢＣＧ）６５ＫＤ热休克蛋白的提纯方法。方法：ＢＣＧ经３７℃恒温振荡培养两周，４２℃热休克处理２ｈ，培养液经离心、抽滤、盐析沉淀、ＳＤＳ－ＰＡＧＥ分离、电泳洗脱等步骤纯化。结果：提纯产物经ＳＤＳ－ＰＡＧＥ分析，其电泳区带在６５ＫＤ位置，经抑制试验表明具有较高抗原活性。结论：流程方法简单、实用，有助于对ＩＤＤＭ的诊断及其深入研究。

结核分枝杆菌HSP65与IL-2融合蛋白的表达和纯化

目的获得融合表达的结核分枝杆菌热休克蛋白65与人白细胞介素2的重组蛋白,为进一步研究其对结核疫苗的作用奠定基础。方法用PCR的方法分别从H37Rv DNA和质粒pGEM-Teasy-IL-2中扩增目的基因片段hsp65和IL-2,将各目的片段克隆至pMD18-T载体中进行测序,将测序正确的目的基因片段分别经EcoRI和ClaI,ClaI和HindⅢ双酶切后亚克隆至原核表达载体pPro-EX HTa,转化大肠杆菌DH5α,挑选阳性克隆,经IPTG诱导后进行融合表达,并通过镍柱对融合蛋白进行纯化。结果PCR法扩增获得的各目的基因片段与GenBank报道的一致。构建的融合蛋白原核表达载体在大肠杆菌中表达后,经SDS-PAGE和Western-blot分析,在Mr 78000处有特异性的蛋白表达条带。用镍柱进行亲和层析纯化后得到了高纯度的HSP65-IL-2融合蛋白。结论成功的构建了结核分枝杆菌HSP65与人IL-2的融合表达载体,并在大肠杆菌中获得高效表达,有望为结核的预防提供有效的疫苗。

热休克蛋白65及其融合蛋白Hsp65-6×P277的分离纯化和稳定性研究(英文)

来源于牛分枝杆菌的热休克蛋白65(Hsp65)在没有佐剂的情况下可作为载体分子将抗原表位递呈给免疫系统。热休克蛋白具有蛋白酶的催化活性,容易发生自溶而降解,这制约了基于Hsp65疫苗的研究。该研究中,建立了纯化Hsp65及其融合蛋白Hsp65-6×P277(P277为来源于人热休克蛋白60的肽段,线性重复6次)的方法。Hsp65与Hsp65-6×P277以可溶形式表达于大肠杆菌。在低温及添加EDTA的条件下经细胞裂解、硫酸铵沉淀及阴离子交换树脂等纯化方法,可得到电泳纯的目的蛋白。用纯化的融合蛋白Hsp65-6×P277免疫小鼠,可激发机体产生强烈的免疫应答,该融合蛋白有希望作为免佐剂的糖尿病疫苗加以进一步研究开发。

皮下免疫热休克蛋白65对高密度脂蛋白抗炎抗氧化功能的影响

目的观察不同剂量热休克蛋白65对载脂蛋白E基因敲除小鼠高密度脂蛋白抗炎抗氧化功能的影响。方法 8周龄载脂蛋白E基因敲除小鼠随机分为磷酸盐缓冲液对照组、5μg热休克蛋白65组及25μg热休克蛋白65组,分别于第3、6周进行皮下免疫。第16周取标本,分别检测血脂水平、血清屏氧酶1活性、髓过氧化物酶活性、高密度脂蛋白炎症指数及炎症因子白细胞介素10和干扰素γ含量。结果随着热休克蛋白65剂量的增加,血清高密度脂蛋白胆固醇水平和白细胞介素10表达量逐渐下降,屏氧酶1活性逐渐降低,高密度脂蛋白炎症指数、髓过氧化物酶活性和干扰素γ表达量则逐渐升高。与对照组比较,25μg热休克蛋白65组血清高密度脂蛋白胆固醇水平和白细胞介素10表达量明显下降(P<0.01),屏氧酶1活性明显降低(P<0.05),高密度脂蛋白炎症指数、髓过氧化物酶活性、干扰素γ表达量则显著升高(P<0.01)。结论热休克蛋白65可引起炎症反应,损害高密度脂蛋白抗炎抗氧化功能,并且这种作用与其剂量有关。

P277多肽融合热休克蛋白65提高抗1型糖尿病的作用

为了提高P277肽抗1型糖尿病的作用,把P277肽融合在卡介苗热休克蛋白65的C端,构建了pET28a- HSP65-P277高效表达载体,在大肠杆菌中高效可溶性表达。利用硫酸铵分级沉淀、阴离子交换柱层析分离纯化了融合蛋白HSP65-P277。使用HSP65-P277在没有任何佐剂存在的情况下免疫非肥胖性糖尿病(NOD)小鼠,通过三次腹腔注射,每月收集被免疫动物的血清,血糖浓度用自动生化分析仪测定。结果显示HSP65-P277免疫组小鼠血糖平均值及糖尿病的累积发病率和其余组相比均有显著差异(P<0.01),融合蛋白HSP65-P277抗NOD小鼠糖尿病的作用显著高于单独的P277和HSP65。为进一步开发能用于临床的1型糖尿病疫苗提供了良好的设计思路,HSP65-P277极有可能进一步发展成为新的抗Ⅰ型糖尿病的疫苗。

重组热休克蛋白65通过鼻黏膜免疫对NOD小鼠胰腺炎和糖尿病发生的影响

目的:研究重组热休克蛋白65通过鼻黏膜免疫途径对NOD小鼠胰腺炎和糖尿病发生的影响。方法:通过PCR方法克隆出结核分枝杆菌的热休克蛋白65的基因序列,构建了pET28a-HSP65高效表达载体,在大肠杆菌中高效可溶性表达,利用阴离子交换柱层析分离纯化。在不添加佐剂的情况下以纯化的HSP65通过3次鼻黏膜免疫非肥胖型1型糖尿病模型动物(NOD)小鼠,每月采集小鼠的血清,通过酶联免疫吸附试验(ELISA)和Western blot检测血清中抗体的产生,利用自动生化分析仪检测血糖浓度。结果:通过鼻黏膜免疫途径可成功诱导小鼠产生特异的抗HSP65抗体,组织病理学分析也显示HSP65通过鼻黏膜免疫能降低NOD小鼠胰腺病变的产生。结论:HSP65通过鼻黏膜免疫能预防NOD小鼠糖尿病的发生,证实了HSP65经鼻黏膜免疫能降低和自身免疫性糖尿病有关的炎症过程的严重性,对1型糖尿病的治疗提供了一个新的途径。

结核杆菌热休克蛋白65“自杀性”DNA疫苗的构建及其免疫效应研究

目的构建表达结核杆菌热休克蛋白65(HSP65)的“自杀性”DNA疫苗。方法用聚合酶链反应,从我室构建的表达结核杆菌HSP65真核表达质粒中(pCHSP65),扩增出编码HSP65的基因,与“自杀性”DNA载体pSFV重组。经酶切、测序鉴定,间接免疫荧光(IF)证实其能表达HSP65后,将此“自杀性”DNA疫苗(pAHSP65)免疫小鼠。用ELISA、MTT法研究其免疫效应,并观察其对结核菌感染小鼠的保护作用。结果酶切、测序鉴定结果证实为结核杆菌HSP65基因,在BHK21细胞中经IF证实有HSP65表达。该疫苗接种能诱导小鼠产生特异性抗体,刺激淋巴细胞增殖,并能抵抗结核杆菌的感染。结论我们成功地构建了表达结核杆菌HSP65的“自杀性”DNA疫苗,该疫苗能诱导特异性免疫应答,并对结核菌感染的小鼠有保护作用。其免疫效应优于常规的HSP65DNA疫苗。

pIHsp65GM的构建及其对结核杆菌感染小鼠的保护

目的构建pIHsp65GM双顺反子真核表达质粒,并在真核细胞中表达,研究该基因疫苗的免疫原性及其对小鼠感染结核杆菌后的免疫保护效果。方法制备基因疫苗,将C57BL/6小鼠于胫前肌注射质粒DNA免疫,末次免疫后用h37rv强毒株经尾静脉攻击小鼠,计数肺和脾组织中结核杆菌的菌落数,对小鼠的部分肺和脾组织作病理切片,经HE染色观察组织病变的程度,测血清特异性IgG,MTT测定脾淋巴细胞特异性增殖指数,测小鼠脾细胞培养上清中IFN-γ的水平,乳酸脱氢酶(LDH)释放法测定免疫小鼠特异性细胞毒性T细胞(CTL)活性。结果 pIHsp65GM基因疫苗构建成功并且诱导小鼠特异性IgG的产生、脾淋巴细胞增殖以及IFN-γ的分泌(平均含量显著高于2个阴性对照组(P<0.001))。pIHsp65GM免疫组小鼠的脾和肺的平均结核菌载量分别低于两个阴性对照组的相应器官的结核菌载量(P<0.001),同时也显著高于BCG免疫对照组。结论成功构建和表达pIHsp65GM质粒,该基因疫苗对小鼠结核杆菌感染有一定的免疫保护效果。

HSP65-MUC1肿瘤疫苗对小鼠胰腺组织的分子模拟作用

目的:探讨重组抗肿瘤融合蛋白疫苗热激蛋白65-黏蛋白1(HSP65-MUC1)在小鼠体内通过分子模拟方式损伤小鼠胰腺的可能性。方法:21只C57BL/6小鼠随机分为PBS对照组、HSP65组和HSP65-MUC1组(每组7只),分别皮下注射PBS、HSP65和HSP65-MUC1,每周1次,给药3周。无菌分离小鼠脾细胞,利用流式细胞术检测特异性淋巴细胞的增殖情况,组织病理学观察小鼠胰腺的病理改变。结果:流式细胞术检测,与PBS对照组和HSP65组比较,HSP65-MUC1肿瘤疫苗组HSP65-MUC1特异性淋巴细胞升高了16.88%(P<0.001);HSP65特异性淋巴细胞升高了7.29%(P<0.01);与HSP60交叉识别的特异性淋巴细胞升高了5.79%(P<0.05)。3个免疫组小鼠胰腺组织HE染色病理均正常。结论:HSP65-MUC1肿瘤疫苗没有通过分子模拟诱导损伤小鼠胰腺。

HTA-HSP70-BCG诱导的DC疫苗体内抗瘤作用的研究

目的:观察HTA-HSP70-BCG诱导的DC疫苗体内抗瘤效应和机制。方法:骨髓来源的不成熟DC通过在培养基中加入rmGM-CSF和rmIL-4培养5天获得。以HTA-HSP70-BCG冲激DC24小时获得DC疫苗,用流式细胞仪检测DC表面CD86和CD40的表达。取健康BALB/c(SPF)小鼠,第0天右腋皮下接种Hca-F细胞,第5天随机分成5组,分别为:①攻击对照组,不进行任何治疗;②CTX化疗组,第5天在接种部位注射CTX;③CTX+不成熟DC组,注射CTX6小时后,于小鼠左腋皮下注射不成熟DC;④CTX+HTA-HSP70-BCG组,注射CTX6小时后,于小鼠左腋皮下注射HTA-HSP70-BCG;⑤CTX+HTA-HSP70-BCGDC组,注射CTX6小时后,于小鼠左腋皮下注射HTA-HSP70-BCG冲激的DC,于第26天解剖小鼠,称瘤重。制备各组小鼠全脾细胞作为效应细胞,以Hca-F瘤细胞为靶细胞,培养72小时,用MTT法测杀瘤活性。结果:DC经HTA-HSP70-BCG冲激后,CD86和CD40上调,分别为98·17%和90·08%(P<0·05),HTA-HSP70-BCGDC组肿瘤的体积和重量均较对照组和其它处理组小(P<0·05),HTA-HSP70-BCGDC组的脾细胞比对照组和其它处理组有较强的杀Hca-F瘤细胞的能力(P<0·05)。结论:体外构建的HTA-HSP70-BCGDC疫苗在小鼠体内可诱导出较强的杀瘤效应。

鼻粘膜免疫融合蛋白Hsp65-6×p277预防NOD小鼠1型糖尿病的发生(英文)

目的提高多肽p277的免疫原性,从而提高其对自身免疫性糖尿病的预防作用。方法将p2776次重复与Hsp65融合置于pET28a中构建重组Hsp65-6×p277表达质粒。该重组质粒在大肠杆菌BL21中以高效可溶形式表达。依次通过细胞裂解、硫酸铵沉淀、双蒸水透析、DEAE纤维素52柱层析纯化获得目的蛋白。用纯化后的融合蛋白Hsp65-6×p277通过鼻腔给药方式,在不添加任何佐剂的情况下3次免疫4周龄雌性NOD小鼠。每月眼角取血,检测抗体和血糖浓度。结果初步药效学实验表明融合蛋白Hsp65-6×p277可抑制NOD小鼠中1型糖尿病的发生。结论融合蛋白Hsp65-6×p277有可能发展成为一种具有防治胰岛素依赖性糖尿病作用的疫苗。

溃疡性结肠炎发病新机制以及热休克蛋白65的作用

溃疡性结肠炎是一种肠道非特异慢性炎症疾病,被世界卫生组织列为难治疾病,目前尚无特效治疗手段.溃疡性结肠炎病因和发病机制尚不十分清楚,限制了治疗药物的开发.对肠道菌群、热休克蛋白家族在溃疡性结肠炎发病中的作用以及热休克蛋白65的潜在治疗作用,以期加深对溃疡性结肠炎发病机制认识,为寻找潜在治疗靶点及药物开发提供借鉴.