AAV mediated carboxyl terminus of Hsp70 interacting protein overexpression mitigates the cognitive and pathological phenotypes of APP/PS1 mice

The E3 ubiquitin ligase,carboxyl terminus of heat shock protein 70(Hsp70)interacting protein(CHIP),also functions as a co-chaperone and plays a crucial role in the protein quality control system.In this study,we aimed to investigate the neuroprotective effect of overexpressed CHIP on Alzheimer’s disease.We used an adeno-associated virus vector that can cross the blood-brain barrier to mediate CHIP overexpression in APP/PS1 mouse brain.CHIP overexpression significantly ameliorated the performance of APP/PS1 mice in the Morris water maze and nest building tests,reduced amyloid-βplaques,and decreased the expression of both amyloid-βand phosphorylated tau.CHIP also alleviated the concentration of microglia and astrocytes around plaques.In APP/PS1 mice of a younger age,CHIP overexpression promoted an increase in ADAM10 expression and inhibitedβ-site APP cleaving enzyme 1,insulin degrading enzyme,and neprilysin expression.Levels of HSP70 and HSP40,which have functional relevance to CHIP,were also increased.Single nuclei transcriptome sequencing in the hippocampus of CHIP overexpressed mice showed that the lysosomal pathway and oligodendrocyte-related biological processes were up-regulated,which may also reflect a potential mechanism for the neuroprotective effect of CHIP.Our research shows that CHIP effectively reduces the behavior and pathological manifestations of APP/PS1 mice.Indeed,overexpression of CHIP could be a beneficial approach for the treatment of Alzheimer’s disease.

Effect of Ultraviolet Radiation on Hsp70 Protein Expression in HaCaT Cells

Ultraviolet radiation by its wavelength is divided into: UVA, UVB and UVC. Only UVA and UVB manage to penetrate the ozone layer, but due to anthropological activities, all of them are capable of interacting with humans to a greater or lesser extent, and can generate adverse effects such as cellular stress when interacting with intra-and extracellular biomolecules. The skin is the first organ in contact with UV radiation, and the stress it generates can be analyzed by the expression of a bioindicator of cellular damage such as Hsp70. Therefore, the objective of the project was: to determine the effect of UVA, UVB and UVC radiation on HaCaT epithelial cells, by analyzing the expression of Hsp70. Materials and methods: HaCaT cells were cultured in vitro, which were irradiated with UVA, UVB and UVC light at different doses, to subsequently determine the degree of Hsp70 expression by Immunodetection by PAGE-SDS and Western Blot. Results: Basal expression of Hsp70 was observed in no irradiated HaCaT cells. When HaCaT cells were irradiated with UVA, UVB, UVC, an increase in this Hsp70 protein was observed. With UVA, a higher degree of expression was observed at a time of 30 minutes of irradiation. With UVB the highest expression shifted to a time of 20 minutes. With UVC, overexpression was observed after 10 minutes. Conclusion: UV radiation generates cellular stress on HaCaT cells, evaluated by the stress bioindicator Hsp70. According to the wavelength of UV radiation, those that have a shorter wavelength have a greater potential for cellular damage, such as UVC.

Novel heat shock protein Hsp70L1 activates dendritic cells and acts as a Th1 polarizing adjuvant

Heat shock proteins (HSPs) are reported to act as effective adjuvants to elicit anti-tumor and anti-infection immunity. Here, we report that Hsp70-like protein 1 (Hsp70L1), a novel HSP derived from human dendritic cells (DCs), has potent adjuvant effects that polarize responses toward Th1. With a calculated molecular weight of 54.8 kDa, Hsp70L1 is smaller in size than Hsp70 but resembles it both structurally and functionally. Hsp70L1 shares common receptors on DCs with Hsp70 and can interact with DCs, promoting DC maturation and stimulating secretion of the proinflammatory cytokines interleukin 12p70 (IL-12p70), IL-1beta, tumor necrosis factor-alpha (TNF-alpha), and the chemokines IP-10, macrophage inflammatory protein-1alpha (MIP-1alpha), MIP-1beta, and normal T cell expressed and secreted (RANTES). The induction of interferon-gamma-inducible protein 10 (IP-10) secretion by Hsp70L1 is not shared by Hsp70, and other functional differences include more potent stimulation of DC IL-12p70, CC-chemokine, and CCR7 and CXCR4 expression by Hsp70L1. Immunization of mice with the hybrid peptide Hsp70L1-ovalbumin(OVA)(257-264) induces an OVA(257-264)-specific Th1 response and cytotoxic T lymphocyte (CTL) that results in significant inhibition of E.G7-OVA tumor growth. The ability of Hsp70L1 to activate DCs indicates its potential as a novel adjuvant for use with peptide immunizations; the Hsp70L1 antigen peptide hybrid may serve as a more effective vaccine for the control of cancer and infectious diseases.

大鼠脑震荡伤后脑组织HSP70、bFGF及TGF-β1表达变化

目的研究脑震荡后脑组织损伤修复相关因子表达变化,为推断脑损伤时间提供法医学依据。方法建立SD大鼠脑震荡伤模型,提取脑组织行常规HE染色及热休克蛋白70(heat shock protein 70,HSP70)、碱性成纤维细胞生长因子(basic fibroblast growth factor,bFGF)和转化生长因子β1(transforming growth factor beta1,TGF-β1)免疫组织化学染色,在光学显微镜下观察并进行图像分析及相应统计学处理。结果伤后30min,在大脑皮质、海马区见少量呈弥散性分布的HSP70免疫组化染色阳性细胞,12h达高峰,伤后1d阳性细胞数量开始减少;伤后3h,在大脑皮质、海马区bFGF免疫组化染色阳性细胞开始增多,至12h时达高峰,然后开始下降;伤后6h～1d,在大脑皮质、海马区TGF-β1免疫组化染色阳性细胞逐渐增多,至3d时达高峰,然后开始下降。结论HSP70、bFGF、TGF-β1在脑震荡后脑组织中表达呈时序性改变。多指标综合应用为法医学损伤时间的推断提供了全新的视角。

针刺对急性高血压脑出血大鼠HSP_(70)表达的良性调整作用

目的 :探索针刺对急性高血压脑出血大鼠治疗作用机制。方法 :复制急性高血压脑出血大鼠模型 ,动态观察针刺对脑组织热休克蛋白 70表达的影响。结果与结论 :针刺能够增加热休克蛋白 70在脑组织中的表达是针刺治疗急性脑出血的一个重要机制。

Graves眼病眼眶组织HLA-DR和HSP-70表达的研究

目的 了解Graves眼病患者眼部组织的组织相容性抗原DR(HLA-DR)和热休克蛋白(HSP-70)的表达极其与病程和治疗的关系。方法 收集Graves眼病患者的眼外肌19例,通过免疫组化的方法观察HLA-DR和HSP-70在不同病程,治疗与未治疗患者眼外肌的表达差异。结果 HLA-DR在眼外肌的纤维母细胞、血管内皮细胞和浸润的淋巴细胞表达,以未治病人的眶组织为明显;HSP-70在肌细胞和纤维母细胞表达,病程短的病人其表达增强。结论 眼外肌细胞和纤维母细胞可能都是Graves眼病自身免疫反应的重要靶细胞;HLA-DR和HSP-70在自身免疫反应中起重要作用;病程和治疗影响HLA-DR和HSP-70的表达。

Aβ_(25～35)诱导阿尔茨海默病模型大鼠海马神经元HSP70的表达

目的利用β淀粉样蛋白(Aβ25～35)毒性作用诱导大鼠阿尔茨海默病(AD)模型,研究热休克蛋白70(HSP70)在海马神经元损伤中的表达。方法将大鼠随机分为2组:AD模型组、溶媒体组,在双侧海马分别注射2μl(10μg)Aβ25～35、2μl生理盐水;于海马注射第1,7,14,21天采用免疫组织化学、积分光密度分析等手段对各组大鼠脑HSP70的表达进行观察。结果AD模型组手术第7天大鼠记忆明显减退(P<0.05),且HSP70在海马神经元内表达第1天时最高,第1～21天呈递减趋势,其中第14天锐减。结论Aβ25～35通过氧化应激和损伤海马神经元等过程使HSP70的表达明显降低,HSP70表达是AD大鼠脑内神经元存活的重要标志。

电击死兔骨骼肌及心肌HSP 70 mRNA和c-fos mRNA表达

目的研究电击死兔骨骼肌与心肌HSP 70 mRNA和c-fos mRNA表达变化,探究生前电击与死后电击的鉴别方法。方法15只新西兰兔,随机分电击死组、死后电击组和对照组,每组5只,用荧光RT-PCR技术检测骨骼肌与心肌热休克蛋白70(HSP 70)mRNA与c-fos mRNA表达水平,对所得结果进行统计学分析。结果生前电击兔骨骼肌及心肌HSP 70 mRNA与c-fos mRNA表达高于死后即刻电击者(P<0.05)。结论检测骨骼肌及心肌HSP 70 mRNA与c-fos mRNA表达变化有助于于生前电击与死后电击的鉴别。

松材线虫Hsp70基因的克隆与原核表达

热激蛋白70（Hsp70）是已知热休克蛋白家族中最重要的一种,它在细胞内的大量表达可以明显改善细胞的生存能力,提高对环境胁迫或伤害的耐受性。采用RACE-PCR技术,从松材线虫（Bursaphelenchus xylophilus）中克隆了Hsp70基因的全长cDNA序列（共2 061 bp）（GenBank登录号为：DQ785812）。其编码一个分子量为70 kD的642个氨基酸的蛋白序列,含有3段Hsp70家族的签名序列。同源性分析表明,氨基酸序列与其它真核生物的Hsp70序列具有很高的相似性,并与秀丽隐杆线虫（Caenorhabditis elegans）热激蛋白70家族中的hsp-1基因编码的氨基酸序列更为相似。因此,将克隆的松材线虫Hsp70基因命名为Bx-hsp-1。构建了一个原核表达载体Bx70pEASY-E1,当IPTG终浓度为0.4-0.8 mmol/L时,能诱导表达融合蛋白。Bx-hsp-1基因的克隆和表达,将为松材线虫的生态适应性机理研究奠定基础。

大鼠局灶性脑缺血再灌注损伤白藜芦醇与HSP70蛋白表达的关系

目的探讨大鼠局灶性脑缺血再灌注损伤白藜芦醇与热休克蛋白(HSP)70的关系和作用。方法随机设立假手术组、对照组和白藜芦醇预处理组3个组,后两组采用线栓法建立大鼠大脑中动脉闭塞模型(MCAO)缺血2 h再灌注,且设立6 h和24 h两个再灌注时间点。白藜芦醇预处理组按40 mg/kg经腹腔注射。分别在术后不同时间点进行神经功能学评分,采用免疫组化和免疫印迹法测定HSP70蛋白表达。结果对照组和白藜芦醇预处理组与假手术组比较神经功能评分显著增高,白藜芦醇预处理组又明显低于对照组(P<0.05);免疫组化和免疫印迹结果一致,对照组和白藜芦醇预处理组与假手术组比较HSP70蛋白表达显著增高,白藜芦醇预处理组HSP70蛋白表达又明显高于对照组(P<0.05)。结论大鼠局灶性脑缺血再灌注损伤白藜芦醇的神经保护作用可以通过热休克蛋白HSP70蛋白的表达增多来产生。

涎腺肿瘤中HSP27、HSP70与PCNA、CD9蛋白表达的相关性

目的研究热休克蛋白(HSP)27和70在涎腺肿瘤中的表达特征及与增殖细胞核抗原(PCNA)和移动相关蛋白-1(MRP-1,CD9)的相关性,探讨其对涎腺肿瘤发生发展的可能作用。方法采用免疫组化SP法和免疫组化双标双染法检测41例良性和17例恶性肿瘤中HSPs的表达。结果 (1)涎腺肿瘤中HSP27和HSP70高表达,但表达定位和强度存在差异。(2)涎腺恶性肿瘤中HSP27和CD9的阳性率和阳性强度均降低(P<0.05和P<0.01)而HSP70和PCNA的阳性率和阳性强度均增高(P均<0.05)。(3)HSP70的阳性率与阳性强度均与PCNA正相关(相关系数分别为Cramer’sV=3797和r=0.5123,P均<0.01);HSP27的表达率与CD9的阳性率正相关(Cramer’sV=0.3477),但阳性强度比较无相关(r=0.1762,P>0.05)。结论 (1)HSP70可能促进PCNA高表达,有用于涎腺肿瘤细胞的增殖。(2)HSP27可能不完全抑制肿瘤细胞的增殖。(3)HSP27和CD9的表达减少均可能是肿瘤细胞分化降低的标志,协同于增殖的恶性肿瘤细胞的迁移。

肿瘤细胞HSP-70多肽诱导CTL及其抗瘤作用机制的研究

目的 探讨鼠S1 80 细胞HSP 70多肽诱导杀伤性T淋巴细胞 (CTL)及其特异性抗瘤作用机制。方法 从 43℃ 9h热休克诱导HSP高表达的S1 80 细胞提纯 80 μg mlHSP 70多肽 ,体外刺激小鼠脾淋巴细胞扩增、活化 ,然后用MTT法测定其杀瘤活性 ,并用电镜观察其培养上清诱导S1 80 细胞的形态学变化。结果 S1 80 细胞HSP 70多肽体外免疫扩增的小鼠脾淋巴细胞对S1 80 和H2 2 细胞的杀瘤率分别为83 .61%和 9.98% ,其培养上清能诱导S1 80 细胞出现程序化死亡的形态学变化。结论 S1 80 细胞HSP 70多肽能剌激小鼠脾淋巴细胞产生特异性杀伤S1 80 细胞的免疫活性细胞 ,该细胞还能分泌免疫活性物质诱导肿瘤细胞凋亡。

HeLa细胞HSP-70多肽体外诱导免疫活性细胞及其抗瘤机理

[目的]探讨用HeLa细胞HSP 70多肽诱导免疫活性细胞 (immunecompetentcells ,ICC)的特异性抗肿瘤机制。[方法]用热休克处理的HeLa细胞提取的HSP 70多肽剌激正常人外周血单个核细胞 ,在剌激扩增前后测定T淋巴细胞表型 ,并测定扩增的免疫活性细胞对HeLa细胞的杀瘤活性。[结果]在扩增的细胞中CD3+、CD8+淋巴细胞百分率明显增高 (P<0.01)。该免疫活性细胞对Hela细胞和来源于病人的宫颈癌细胞都具有较高的杀伤活性 ,而对经HSP 70单抗封闭后的HeLa细胞的杀伤率则明显下降。[结论]HeLa细胞HSP 70多肽能有效刺激PBMCs诱导活化免疫活性细胞 。

热休克蛋白Hsp70在抗原呈递过程中的作用

目的研究热休克蛋白Hsp70家族在抗原呈递中的作用,探讨其与肿瘤免疫反应的关系。方法利用反义RNA技术,将反义Hsp70、反义Hsc70、B7表达质粒导入肿瘤细胞B16中,24 h后检测细胞中热休克蛋白表达水平。利用混合淋巴细胞培养,检测T淋巴细胞增殖能力。结果在黑色素瘤细胞B16中转染pLXSN-antihsp70、pLXSN-antihsc70及2者共转染,转染反义质粒能够抑制B16细胞中Hsp70/Hsc70的表达,导致Hsp70表达下调,其刺激T淋巴细胞增殖能力均大幅下降。而将pLXSNmB7转染入B16细胞中,其刺激T细胞增殖的能力均有所上升。转染pLXSNmB7后,B16细胞中Hsp70/Hsc70的表达量有所提高。结论抑制各热休克蛋白Hsp70家族的表达能够导致T细胞增值数降低。在肿瘤细胞中导入B7分子能够提高Hsp70的表达水平,从而提高其抗原呈递的能力。

Purification of heat shock protein 70-associated tumor peptides and their antitumor immunity to hepatoma in mice

AIM:To purify the heat shock protein (HSP) 70-associated tumor peptides and to observe its non-MHC-I molecule restrictive antitumor effect.METHODS:By ConA-sepharose affinity chromatography,ADP-agarose affinity chromatography, and DEAE anion exchange chromatography, we were able to purify HSP70-associated peptides from mouse hepatoma (HCaF) cells treated in heat shock at 42℃. Specific active immunization and adoptive cellular immunization assay were adopted to observe the immunoprotective effect elicited by HSP70-associated peptide complexes isolated from HcaF.RESULTS: The finally purified HSP-associated peptides had a very high purity and specificity found by SDS-PAGE and Western blot. Mice immunized with HSP70-associated peptide complexes purified from HCaF cells were protected from HCaF living cell challenge. This effect was dose dependent.Adoptive immunization of immune spleen cells of mice immunized with HSP70-associated peptide complexes could elicit immunity against HCaF challenge, and the tumor-free mice could resist repeated challenges. This effect could be continuously enhanced by repeated challenge with HCaF living cells. The tumor-free mice could tolerate the challenge for as high as 1×10^7 HCaF cells. The mice immunized once with spleen cells pulsed with HSP70-associated peptide complexes in vitro could also result in a certain adoptive immunity against HCaF.CONCLUSION:High purity and specificity of HSP70-associated peptides could be achieved from tumor cells by the low-pressure affinity chromatography method used in this study. HSP70-associated peptide complexes derived from the HCaF can elicit non-MHC-I molecule restrictive immunoprotective effect against HCaF.This effect can be transferred by adoptive immunization to mice and enhanced by repeated challenge with HCaF live cells.

Sleep deprivation increase the expression of inducible heat shock protein 70 in rat gastric mucosa

AIM: To investigate if sleep deprivation is able to increase the expression of inducible heat shock protein 70 in gastric mucosa and its possible role in mucosal defense. METHODS: Rats for sleep disruption were placed inside a computerized rotating drum, gastric mucosa was taken from rats with 1, 3 and 7d sleep deprivation. RT-PCR, immunohistochemistry and Western blotting were used to determine the expression of heat shock protein 70. Ethanol (500mL.L(-1), i.g.) was used to induce gastric mucosa damage. RESULTS: RT-PCR, Western blotting and immunostaining confirmed that the sleep deprivation as a stress resulted in significantly greater expression of inducible heat shock protein 70 in gastric mucosa of rats. After the 500mL.L(-1) ethanol challenge, the ulcer area found in the rats with 7d sleep deprivation (19.15 +/- 4.2)mm(2) was significantly lower (P【0.01) than the corresponding control (53.7 +/- 8.1) mm(2). CONCLUSION: Sleep deprivation as a stress, in addition to lowering the gastric mucosal barrier, is able to stimulate the expression of inducible heat shock protein 70 in gastric mucosa of rats, the heat shock protein 70 may play an important role in gastric mucosal protection.

Effects of Batroxobin on Spatial Learning and Memory Disorder of Rats with Temporal Ischemia and the Expression of HSP32 and HSP70

The effect of Batroxobin on spatial memory disorder of left temporal ischemic rats and the expression of HSP32 and HSP70 were investigated with Morri`s water maze and immunohistochemistry methods. The results showed that the mean reaction time and distance of temporal ischemic rats in searching a goal were significantly longer than those of the sham-operated rats and at the same time HSP32 and HSP70 expression of left temporal ischemic region in rats was significantly increased as compared with the sham-operated rats. However, the mean reaction time and distance of the Batroxobin-treated rats were shorter and they used normal strategies more often and earlier than those of ischemic rats. The number of HSP32 and HSP70 immune reactive cells of Batroxobin-treated rats was also less than that of the ischemic group. In conclusion, Batroxobin can improve spatial memory disorder of temporal ischemic rats; and the down-regulation of the expression of HSP32 and HSP70 is probably related to the attenuation of ischemic injury.

严重创伤早期大鼠下丘脑HSP70与iNOS表达与分布的时效关系

目的 研究严重创伤早期大鼠下丘脑热休克蛋白 (HSP) 70与诱导型一氧化氮合酶 (iNOS)转录表达变化分布和意义。方法 采用BIM Ⅲ型生物撞击机致大鼠胸部严重撞击伤 ,并造成单侧股骨骨折 ,运用S ABC免疫组化、原位杂交技术测定下丘脑HSP70与iNOS及其mRNA的转录表达水平。结果 正常对照组HSP70低水平表达 ,在伤后 1小时即开始明显增高 (P <0 .0 5 ) ,6小时达到峰值为正常的 18倍 ,12小时后开始下降 ,2 4小时时主要集中在室旁核内 ;iNOS无基础表达 ,在伤后 1小时开始出现 ,随HSP70同步增高 ,8小时达到高峰 ,较 1小时时增加 13倍。两者相关系数r =0 .976 0 1。结论 严重创伤后早期下丘脑内HSP70和iNOS过度表达 ,在严重创伤应激时下丘脑的损伤与抗损伤机制中起重要作用。

HSP70与PCNA在中耳胆脂瘤中的表达与意义

目的通过分析热休克蛋白(heat shock protein,HSP)70和增殖细胞核抗原(proliferating cell nuclearantigen,PCNA)蛋白表达的相关性探讨HSP 70在中耳脂瘤病理过程中的可能作用。方法用HSP 70和PCNA单克隆抗体采用SP免疫组织化学方法对21例中耳胆脂瘤石蜡标本进行研究,11例正常外耳道皮肤做为对照。结果与正常外耳道皮肤相比,HSP70和PCNA相关蛋白在中耳胆脂瘤的表达均显著增强,均为P<0.01,二者的表达指数有一定相关性,r=0.568,P<0.01。结论 HSP 70在中耳胆脂瘤的异常表达说明其在胆脂瘤的发生、发展过程中可能有重要作用。HSP 70表达增多的同时胆脂瘤上皮细胞增生程度加重,提示HSP 70可能参与诱导上皮细胞增殖。

Cytotoxic T-lymphocytes response in vitro activated by dendritic cells pulsed with heat shock protein 70 derived from human bladder tumor cell lines of EJ

Objective： To investigate whether human dendritic cells （DC） derived from peripheral blood mononuclear cells （PBMC）, which were pulsed by heat shock protein 70 （HSP70） isolated from human bladder tumor cell lines of E J, were able to induce peptide specific cytotoxic T-lymphocytes （CTL） response in vitro and give the experimental foundation for the future clinical trials of immunotherapy in bladder tumor. Methods： The E J-derived HSP70 co-cultured with DC from the healthy volunteers＇ PBMC, along with the crude lysate （the supematant before HSP70 purification） from EJ cells were used as the experimental groups and DC not pulsed by any tumor cells antigen were the blank control. The autologous T-lymphocytes were added into the above various DC groups, and after incubation, the stimulation indexes （SI） and interferon-y （IFN-γ） were detected to evaluate the immune activities of various DC groups. The killing effects of CTL to target cells, EJ and Hela cells, were determined with 51^Cr releasing test. Results： Both DC/HSP70 and DC/the crude lysate could effectively activate CTL in vitro and kill target cells EJ. The killing effect of DC/HSP70 to EJ was much stronger than DC/the crude lysate （the supernatant before HSP70 purification） （P 〈 0.05）. DC without any tumor cell antigens had a lower killing power to EJ. Meanwhile, DC/ HSP70 had little killing power to Hela non-relevant to bladder tumor histopathologically as compared with EJ cells （P 〈 0.05）. Conclusion： The DC pulsed by HSP70 derived from the autologous tumor cells could induce a peptide complexes specific CTL response to tumor cells, and the CTL response induced by the DC/HSP70 was stronger, which display the basis of the possible clinical application of DC/HSP70 for bladder tumor.