Nmi interacts with Hsp105β and enhances the Hsp105β-mediated Hsp70 expression

The mammalian stress protein Hsp105α is expressed constitutively and is further induced under stress conditions, whereas the alternative spliced form, Hsp105β is only expressed during mild heat shock. We previously reported that Hsp105α is localized mainly in the cytoplasm, whereas Hsp105β is localized in the nucleus. Consistent with the different localization of these proteins, Hsp105β but not Hsp105α induces the expression of the major stress protein Hsp70. We here identified N-myc and Stat interactor (Nmi), as an Hsp105β-binding protein by yeast two-hybrid screening. Immunoprecipitation and pull-down assay showed that Nmi interacts with Hsp105β in vivo and in vitro. Luciferase reporter gene assay and Western blotting showed that Nmi enhanced both the Hsp105β-induced phosphorylation of Stat3 and the Hsp105β-induced activation of the hsp70 promoter in a manner that is dependent on the Stat3-binding site, which results in an increase in Hsp70 protein levels. Most importantly, mild heat shock-induced Hsp70 expression, which is dependent on Hsp105β, is suppressed by knockdown of endogenous Nmi. These results suggest that Nmi has a role as a positive regulator of Hsp105β-mediated hsp70 gene expression along the Stat3 signaling pathway.     

真菌Hsp90研究进展

近年来,随着广谱抗生素、化疗以及器官移植技术的广泛应用,真菌感染日益严重,从分子水平揭示病原真菌的致病机制对真菌感染的防控、治疗至关重要。微生物适应宿主微环境压力的能力在其共生与感染过程中发挥着关键作用,heat shock protein 90（Hsp90）是真核生物参与压力应答响应的分子伴侣,它不仅参与胞内蛋白质的折叠,还与许多底物蛋白相互作用共同调节病原真菌的形态发育、生物被膜形成、有性生殖、毒力以及耐药性。本文从真菌Hsp90的活性调节、底物蛋白,以及Hsp90与病原真菌形态发生、有性生殖、耐药性调控等方面综述了近年来真菌Hsp90信号通路的研究进展。     

重组结核分枝杆菌Hsp16.3的纳米金免疫传感器检测Hsp16.3抗体

克隆和表达结核分枝杆菌热休克蛋白16.3(Hsp16.3),建立纳米金免疫传感器检测结核病患者血清Hsp16.3抗体。PCR扩增hsp16.3基因,构建重组表达质粒pQE30-hsp16.3,表达和纯化Hsp16.3,Western blot分析其反应原性;晶种生长法制备金纳米棒并连接Hsp16.3,建立纳米金免疫传感器检测血清Hsp16.3抗体,接受者操作特性(ROC)曲线评价其灵敏度和特异性。成功构建重组表达质粒pQE30-hsp16.3,纯化Hsp16.3具有良好的反应原性;Hsp16.3的纳米金免疫传感器分别检测50例结核病患者、42例非结核肺病患者和50例体检健康者血清,红移值大于3.5的例数分别为42、7、1例;ROC曲线显示,曲线下面积0.888(P0.01),界值3.5,灵敏度82%,特异性98%。结果表明,Hsp16.3的纳米金免疫传感器可用于检测结核病血清Hsp16.3抗体。     

Hsp90抑制剂的研究进展

热激蛋白90(heat shock protein90,Hsp90)作为分子伴侣在调节细胞生长、分化、凋亡等方面发挥着重要的作用。Hsp90抑制剂能与Hsp90结合,使其功能丧失,造成细胞的多种生理活动缺陷,在Hsp90功能研究和癌症治疗方面具有潜在的价值。综述了不同来源的Hsp90抑制剂及其作用机制,同时对新型Hsp90抑制剂的来源进行了探讨。     

The atheroprotective properties of Hsp70: a role for Hsp70-endothelial interactions?

Although heat shock (stress) proteins are typically regarded as being exclusively intracellular molecules, it is now apparent that they can be released from cells in the absence of cellular necrosis. We and others have reported the presence of Hsp60 (HSPD1) and Hsp70 (HSPA1A) in the circulation of normal individuals and our finding that increases in carotid intima-media thicknesses (a measure of atherosclerosis) in subjects with hypertension at a 4-year follow-up are less prevalent in those having high serum Hsp70 (HSPA1A) levels at baseline suggests that circulating Hsp70 (HSPA1A) has atheroprotective effects. Given that circulating Hsp70 (HSPA1A) levels can be in the range which has been shown to elicit a number of biological effects in vitro, and our preliminary findings that Hsp70 (HSPA1A) binds to and is internalised by human endothelial cell populations, we speculate on the mechanisms that might be involved in the apparent atheroprotective properties of this protein.     

Hsp70在病毒复制中的作用

热休克蛋白70(Heat shock protein 70, Hsp70)是一种在进化上高度保守的分子伴侣蛋白,参与蛋白质的合成、折叠、组装及降解等过程,还参与细胞抗逆境胁迫的响应,对细胞蛋白内稳态（Protein homeostasis）的维持和生物体健康具有重要作用。研究表明,Hsp70对病毒的感染和复制也发挥重要作用。本文就Hsp70的结构、Hsp70对病毒复制的促进及抑制作用进行综述,以期更深入地阐明Hsp70发挥作用的分子机制并为寻找以Hsp70为靶点的抗病毒药物提供新的理论依据及思路。     

Hsp60 and Hsp10 increase in colon mucosa of Crohn’s disease and ulcerative colitis

The purpose of this work was to determine in colon mucosa of Crohn’s disease (CD) and ulcerative colitis (UC) in relapse: a) the levels of the chaperonins Hsp60 and Hsp10; b) the quantity of inflammatory cells; and c) if the levels of chaperonins parallel those of inflammation cells. Twenty cases of CD and UC and twenty normal controls (NC) were studied using immunohistochemistry, Western blotting and immunofluorescence. Immunohistochemically, Hsp60 and Hsp10 were increased in both inflammatory bowel diseases (IBD) compared to NC. These results were confirmed by Western blotting. Hsp60 and Hsp10 occurred in the cytoplasm of epithelial cells in CD and UC but not in NC. Hsp60 and Hsp10 co-localised to epithelial cells of mucosal glands but not always in connective tissue cells of lamina propria, where only Hsp60 or, less often, Hsp10 was found. Cells typical of inflammation were significantly more abundant in CD and UC than in NC. Since chaperonins are key factors in the activation of the immune system leading to inflammation, we propose that they play a central role in the pathogenesis of the two diseases, which, consequently, ought to be studied as chaperonopathies.     

Substitution of only two residues of human Hsp90α causes impeded dimerization of Hsp90β

Two isoforms of the 90-kDa heat-shock protein (Hsp90), i.e., Hsp90α and Hsp90β, are expressed in the cytosol of mammalian cells. Although Hsp90 predominantly exists as a dimer, the dimer-forming potential of the β isoform of human and mouse Hsp90 is less than that of the α isoform. The 16 amino acid substitutions located in the 561–685 amino acid region of the C-terminal dimerization domain should be responsible for this impeded dimerization of Hsp90β (Nemoto T, Ohara-Nemoto Y, Ota M, Takagi T, Yokoyama K. Eur J Biochem 233: 1–8, 1995). The present study was performed to define the amino acid substitutions that cause the impeded dimerization of Hsp90β. Bacterial two-hybrid analysis revealed that among the 16 amino acids, the conversion from Ala₅₅₈ of Hsp90β to Thr₅₆₆ of Hsp90α and that from Met₆₂₁ of Hsp90β to Ala₆₂₉ of Hsp90α most efficiently reversed the dimeric interaction, and that the inverse changes from those of Hsp90α to Hsp90β primarily explained the impeded dimerization of Hsp90β We conclude that taken together, the conversion of Thr₅₆₆ and Ala₆₂₉ of Hsp90α to Ala₅₅₈ and Met₆₂₁ is primarily responsible for impeded dimerization of Hsp90β.     

Combination of Correctors Rescue ΔF508-CFTR by Reducing Its Association with Hsp40 and Hsp27

Correcting the processing of ΔF508-CFTR, the most common mutation in cystic fibrosis, is the major goal in the development of new therapies for this disease. Here, we determined whether ΔF508 could be rescued by a combination of small-molecule correctors, and identified the mechanism by which correctors rescue the trafficking mutant of cystic fibrosis transmembrane conductance regulator (CFTR). We transfected COS-7 cells with ΔF508, created HEK-293 stably expressing ΔF508, and utilized CFBE41o⁻ cell lines stably transduced with ΔF508. As shown previously, ΔF508 expressed less protein, was unstable at physiological temperature, and rapidly degraded. When the cells were treated with the combination C18 + C4 the mature C-band was expressed at the cell surface. After treatment with C18 + C4, we saw a lower rate of protein disappearance after translation was stopped with cycloheximide. To understand how this rescue occurs, we evaluated the change in the binding of proteins involved in endoplasmic reticulum-associated degradation, such as Hsp27 (HspB1) and Hsp40 (DnaJ). We saw a dramatic reduction in binding to heat shock proteins 27 and 40 following combined corrector therapy. siRNA experiments confirmed that a reduction in Hsp27 or Hsp40 rescued CFTR in the ΔF508 mutant, but the rescue was not additive or synergistic with C4 + 18 treatment, indicating these correctors shared a common pathway for rescue involving a network of endoplasmic reticulum-associated degradation proteins.     

TPR蛋白对Hsp90功能的调节

热激蛋白Hsp90是一类在进化中形成的高度保守的且可参与多种细胞功能的特异分子伴侣。TPR蛋白通常存在于Hsp90的多蛋白质复合物中,它对Hsp90的功能的多样性起着至关重要的作用,同时Hsp90可能为TPR蛋白提供“泊位”,允许不同的TPR蛋白在Hsp90分子伴侣底物附近有序而特异结合,从而使Hsp90在细胞内环境中以特定的方式完成其各种细胞功能。了解TPR蛋白与Hsp90的相互作用机制为阐明细胞内Hsp90的功能多样性和特异性奠定了基础。     

Hsp提高细菌的逆境生存能力和乙醇产量

目的：用热休克蛋白Hsp（HeatShockProteins）基因重组大肠杆菌,改善细胞生长状况、提高大肠杆菌的逆境耐受性和乙醇产量。方法：将来自Pyrococcus加诬凇的基因Hsp与Lac启动子串联,构建成由Lae启动子调控Hsp表达的操纵子,经该操纵子转化的大肠杆菌分别在高渗透压、酸性条件、高温和高糖的条件下发酵,利用气相色谱检测发酵液中的乙醇含量。结果：含有Hsp基因的工程菌与不含Hsp基因的对照菌相比,在0．4mol／LNaCl的高渗透压下乙醇产量提高1．5倍、在pH4．5的酸性条件下提高1．2倍、在高温高糖的条件下提高5．95倍。结论：热休克蛋白Hsp基因的表达可以提高大肠杆菌在逆境中的代谢能力。     

Structures of Hsp90α and Hsp90β bound to a purine-scaffold inhibitor reveal an exploitable residue for drug selectivity

Hsp90α and Hsp90β are implicated in a number of cancers and neurodegenerative disorders but the lack of selective pharmacological probes confounds efforts to identify their individual roles. Here, we analyzed the binding of an Hsp90α-selective PU compound, PU-11-trans, to the two cytosolic paralogs. We determined the co-crystal structures of Hsp90α and Hsp90β bound to PU-11-trans, as well as the structure of the apo Hsp90β NTD. The two inhibitor-bound structures reveal that Ser52, a nonconserved residue in the ATP binding pocket in Hsp90α, provides additional stability to PU-11-trans through a water-mediated hydrogen-bonding network. Mutation of Ser52 to alanine, as found in Hsp90β, alters the dissociation constant of Hsp90α for PU-11-trans to match that of Hsp90β. Our results provide a structural explanation for the binding preference of PU inhibitors for Hsp90α and demonstrate that the single nonconserved residue in the ATP-binding pocket may be exploited for α/β selectivity.     

玉米细胞质分子伴侣Hsp70的ATPase活性

玉米胚乳细胞中纯化的细胞质Ｈｓｐ７０蛋白有低水平的ＡＴＰａｓｅ 活性,它在５０ ℃、ｐＨ５ ．８ 、２０ ｍｍｏｌ／Ｌ的ＫＣｌ 条件下活性最高,Ｃａ２＋和Ｍｇ２＋ 抑制其活性。大肠杆菌ＤｎａＪ蛋白能将玉米细胞质Ｈｓｐ７０ 的ＡＴＰａｓｅ 活性提高６倍,而ＧｒｐＥ 蛋白对其影响很小。８ 种不同的人工合成多肽均能刺激该蛋白的ＡＴＰａｓｅ 活性,增加幅度从２ ．５ 倍到１０ 倍不等。亲水性不同的氨基酸对Ｈｓｐ７０ 的ＡＴＰａｓｅ 活性影响不同。玉米细胞质Ｈｓｐ７０ 是一个三磷酸核苷酸酶,除ＡＴＰ 外,它还能催化ＵＴＰ、ＧＴＰ、ＣＴＰ和ＩＴＰ的水解     

Hsp90分子抑制剂拮抗肿瘤耐药的研究进展

Hsp90作为热休克蛋白家族中的重要一员,是一种对细胞生存所必需的分子伴侣,它发挥着稳定顾客蛋白构象、维持其功能的作用。许多顾客蛋白在肿瘤中处于过度表达或持续激活状态,与肿瘤的发生发展有着密切的关系。因此,Hsp90在近年的研究中倍受关注,已经发展为抗肿瘤治疗的良好靶点,目前已经有多个Hsp90抑制剂进入临床实验。近年随着肿瘤分子生物学的研究,肿瘤分子靶向治疗已取得明显成果,针对多种癌症已获得了多个用于靶向治疗的单克隆抗体或小分子化学物质,如用于治疗某些HER2阳性乳腺癌的曲妥珠单抗、用于治疗NSCLC的吉非替尼等。然而随着这些药物的应用,肿瘤耐药性不可避免的产生。多方面研究表明Hsp90抑制剂会引起与耐药相关的多个分子的降解,提示其在拮抗耐药方面具有重要的意义。本文就Hsp90分子抑制剂在拮抗肿瘤耐药方面的研究进行综述。     

玉米细胞质分子伴侣Hsp70的ATPase活性

玉米胚乳细胞中纯化的细胞质Ｈｓｐ７０蛋白有低水平的ＡＴＰａｓｅ活性,它在５０℃、ＰＨ５．８、２０ｍｍｏｌ／Ｌ的ＫＣｌ条件下活性最高,Ｃａ＾２＋和Ｍｇ＾２＋抑制其活性。大肠杆菌ＤｎａＪ蛋白能将玉米细胞质Ｈｓｐ７０的ＡＴＰａｓｅ活性提高６倍,而ＧｒｐＥ蛋白对其影响很小。８种不同的人工合成多肽均能刺激该蛋白折ＡＴＰａｓｅ活性,增加幅度从２．５倍到１０倍痫水性不同的氨基酸对Ｈｓｐ７０的ＡＴＰａｓｅ活性影响