Molecular Cloning the Gene of Small Heat Shock Protein in the Mitochondria and Endoplasmic Reticulum of Tomato

A cDNA Library was constructed with the heat shocked tomato ( Lycopersicon esculentum Mill.) flowers and then was screened with the probes of mitochondrial and endoplasmic reticulum conservative regions that were cloned by using RT-PCR. The complete cDNAs of mitochondrial and endoplasmic reticulum small heat shock protein ( shsp) were selected out from the cDNA library. Furthermore, the temperature responses of these shsp genes were determined. Northern hybridization showed that the heat response temperatures of both genes in tomato flower were lower than that in leaf and that mitochondria shsp in leaf was cold-inducible. In this paper, the molecular features of the cloned genes, the causes of the uncommon heat response temperatures of sHSP in newer and the cold inducible character of mitochondria shsp gene in leaf were discussed.

Expression profiles of two small heat shock proteins and antioxidant enzyme activity in Mytilus galloprovincialis exposed to cadmium at environmentally relevant concentrations

Small heat shock proteins encompass a widespread but diverse class of proteins, which play key roles in protecting organisms from various stressors. In the present study, the full-length cDNAs of two small heat shock proteins （MgsHSP22 and MgsHSP24.1） were cloned from Mytilus galloprovincialis, which encoded peptides of 181 and 247 amino acids, respectively. Both MgsHSP22 and MgsHSP24.1 were detected in all tissues examined by real-time PCR, with the highest expression being observed in muscle and gonad tissues. The real-time PCR results revealed that Cd significantly inhibited MgsHSP22 expression at 24 h and MgsHSP24.1 at 24 and 48 h under 5 ug/L Cd2＋ exposure. MgsHSP24.1 expression was also significantly inhibited after 50 ug/L Cd2＋ exposure for 48 h. With regard to antioxidant enzymes, increased GPx and CAT activity were detected under Cd2＋ stress （5 and 50 ug/L）, while no significant difference in SOD activity was observed throughout the experiment. Overall, both MgsHsps and antioxidant enzymes revealed their potential as Cd stress biomarkers in M. galloprovincialis.

Expression analysis of two reverse duplicated small heat shock protein genes in rice(Oryza sativa L.)

supported by grants from the National Natural Science Foundation of China （30671178）;the Shanxi Province Science Foundation for Youths, China （2014021029-2）

Bioinformatic analysis of embryo development related small heat shock protein Hsp26 in Artemia species

Artemia embryos can endure extreme temperature, long-term anoxia, desiccation and other wide variety of stressful conditions. How the embryos survive these stresses is a very interesting and unsolved subject. To solve this question we analyzed the nucleotide and deduced protein sequence for Hsp26, a molecular chaperone specific to Artemia embryo development, cDNAs of Hsp26 were sequenced from eight Artemia species and deduced Hsp26 amino acid sequences were analyzed. Computer-assisted analysis indicated that the 5＇-untranslated region and all the 3 introns contain many putative cis-acting elements for Hsp26 gene expression during development, including heat shock elements （HSEs）, Dfd, dl, CF2-II, Hb and AP-1 binding sites. Secondary structure of the Hsp26 3＇-untranslated terminator contains the basic structure basis for transcriptional termination. Hsp26 shares sequence similarity with sHSPs （small heat shock protein） from other organisms. The physico-chemical properties of the deduced protein, such as theoretical molecular weight, protein extinction coefficient, isoelectric point and antigenic sites were also obtained. One seven-peptide nuclear localization signals （NLS） ＂PFRRRMM＂ was found, which suggested that the Hsp26 protein was hypothesized to be located inside the nucleus. The numbers of phosphorylation sites of serine, threonine and tyrosine and kinase specific phosphorylation sites are also located in Hsp26 protein sequence. These studies will help us achieve a better understanding of Hsp26 and broad implications for sHSPs function in crustacean embryo development.

Heat Treatment of Small Heat Shock Proteins α-Crystallin and Hsp16.3: Structural Changes vs. Chaperone-like Activity

Both α crystallin from bovine eye lens and Hsp16.3 from Mycobacterium tuberculosis are members of the small heat shock protein family. They were preincubated at 100 ℃ for 15 min and then cooled on ice immediately. The chaperone like activities of preheated proteins were measured at 37 ℃ using DTT treated insulin B chains as substrates. Both preheated proteins exhibited greatly enhanced chaperone like activities, accompanied with almost unchanged secondary structures and surface hydrophobicity but with a minor change in tertiary structures. The dramatically enhanced chaperone like activities of preheated α crystallin and Hsp16.3 may have resulted from the irreversible change in the tertiary structure as detected by near UV CD spectra.

Expression of Heat Shock Protein 70 and 27 in Non-small Cell Lung Cancer and Its Clinical Significance

The heat shock proteins （HSPs） 70 and HSP 27 expression in patients with non-small cell lung cancer （NSCLC） was studied and the relation.ship between HSP 70 and HSP 27 with the clinicopathological features of NSCLC was investigated. The expression of HSP 70 and HSP 27 was detected in tumor tissues from 60 patients with NSCLC by S-P immunohistochemistry. The findings were analyzed in combination with the histological types, histopathological differentiation, lymph node metastasis, patients＇ clinical stages, smoking history and gender. The results showed that of the 60 NSCLC tissue specimens studied, the immunoreactivity of HSP 70 and HSP 27 was detected in 47 （78.3 %） and 43 （71.7 %） specimens, respectively. A positive correlation was found between the overexpression of HSP 70 and HSP 27. The histopathological differentiation, lymph node metastasis, clinical stages and smoking history were correlated to the expression of HSP 70, but not to the expression of HSP 27. No statistical significance was observed in histological types and gender with respect to both HSP 70 and HSP 27 expression. It is suggested that the HSP 70 expression is a powerful and significant prognostic indicator and is related to histopathological differentiation, lymph node metastasis, patients＇ clinical stages, smoking history, whereas HSP 27 expression is not.

小地老虎AiHSP19.3基因鉴定及其对高温和杀虫剂胁迫的响应

小地老虎Agrotis ipsilon是一种重要的农业害虫。小分子热激蛋白(sHSP)是细胞抵御外界胁迫的关键蛋白,本文旨在探索sHSP基因在小地老虎不同发育阶段以及在高温和杀虫剂胁迫下的响应模式。使用同源检索方法从小地老虎转录组中鉴定到了一个sHSP基因的cDNA序列,命名为AiHSP 19.3。通过RT-PCR技术克隆该序列,利用实时荧光定量PCR技术分析AiHSP 19.3基因在小地老虎不同发育阶段和不同组织中的转录模式,并分析了该基因在高温和杀虫剂胁迫下的转录水平。结果表明,小地老虎AiHSP 19.3基因的开放阅读框为516 bp,编码含171个氨基酸,分子量为19.3 kD的蛋白,具有sHSP典型的α-晶状体结构域(ACD)。在供试小地老虎的不同发育阶段和3龄幼虫组织中均能检测到AiHSP 19.3的转录,其中在6龄幼虫和3龄幼虫脂肪体内转录水平最高。小地老虎幼虫经高温和3种杀虫剂(高效氯氟氰菊酯、氯虫苯甲酰胺及辛硫磷)处理后AiHSP 19.3的转录水平显著提高,表明该基因可能在响应高温及杀虫剂胁迫中起到重要作用。

小分子热激蛋白在植物应对高温胁迫中的作用

小分子热激蛋白(sHSPs)是一类不依赖于腺嘌呤核苷三磷酸并具有分子伴侣功能的功能保守型蛋白质。sHSPs在植物受到高温胁迫时产生的热激反应中尤为重要,通过防止错误蛋白质的热集聚、与其他热激蛋白互作,促使错误蛋白质被降解或重新折叠,进而帮助植株响应高温。同时,sHSP的表达受到热休克元件、热休克转录因子、长链非编码RNA(lncRNA)、小分子RNA(miRNA)及一些植物激素的调控。本文总结了植物sHSPs结构功能、调控机制及相关研究进展,着重阐述了植物sHSPs在高温胁迫下的响应机制,为研究植物响应高温的机制提供参考。

血清HSP90α联合lncRNA SNHG5与常规血清肿瘤标志物诊断早期结直肠癌的价值

目的比较血清热休克蛋白90α(HSP90α)联合清长链非编码RNA小核仁RNA宿主基因5(lncRNA SNHG5)和常规血清肿瘤标志物诊断早期结直肠癌(CRC)的临床应用价值。方法采用倾向性评分匹配法和1∶1∶1原则选取2021年3月至2024年4月河南大学第一附属医院收治的215例早期CRC患者(肠癌组)、215例结直肠良性病变患者(良性组)和215例健康体检人群(对照组)作为研究对象。比较三组受检者常规血清肿瘤标志物[癌胚抗原(CEA)、糖类抗原(CA)199、CA242、CA724、CA153、CA50、CA125]、血清HSP90α、lncRNA SNHG5水平,采用受试者工作特征(ROC)曲线及曲线下面积(AUC)分析常规血清肿瘤标志物、血清HSP90α、lnc RNA SNHG5诊断早期CRC的价值,并比较不同方案的诊断效能。结果肠癌组患者的CEA、CA199、CA242、CA724、CA153、CA50、CA125分别为(5.32±1.76)ng/mL、(32.98±10.89)U/mL、(16.19±5.38)U/mL、(8.30±2.72)U/mL、(20.43±6.80)U/mL、(23.79±7.91)U/mL、(40.57±13.25)U/mL,良性组分别为(2.91±0.94)ng/mL、(13.60±4.17)U/mL、(4.79±1.58)U/mL、(3.94±1.00)U/mL、(11.02±3.57)U/mL、(4.46±1.39)U/mL、(40.57±13.25)U/mL,对照组分别为(2.60±0.81)ng/mL、(12.84±3.95)U/mL、(4.25±1.86)U/mL、(3.59±1.16)U/mL、(10.86±3.49)U/mL、(4.15±1.28)U/mL、(14.99±4.95)U/mL,肠癌组患者的上述各项指标明显高于良性组和对照组,差异均有统计学意义(P<0.05),良性组与对照组比较差异均无统计学意义(P>0.05);肠癌组患者的HSP90α、lncRNA SNHG5分别为(34.69±11.50)U/mL、2.84±0.93,良性组分别为(15.30±3.49)ng/L、1.95±0.67,对照组分别为(11.57±2.36)ng/L、1.86±0.51,肠癌组患者的上述各项指标明显高于良性组和对照组,差异均有统计学意义(P<0.05),良性组患者的血清HSP90α水平明显高于对照组,差异均有统计学意义(P<0.05),但良性组和对照组的血清lncRNA SNHG5水平比较差异无统计学意义(P>0.05);ROC分析结果显示,常规血清肿瘤标志物诊断早期CRC的AUC均大于0.75,CEA的AUC和敏感度最高,CA199的特异度最高,CEA+CA199的AUC为0.922,高于其余常规血清肿瘤标志物(P<0.05);HSP90α+lncRNA SNHG5联合诊断早期CRC的AUC为0.943,高于HSP90α、lncRNA SNHG5单独诊断(P<0.05);HSP90α的AUC与CEA、CA199比较差异无统计学意义(P>0.05),lncRNA SNHG5与CEA、CA199比较差异无统计学意义(P>0.05),HSP90α+lncRNA SNHG5的AUC高于CEA+CA199,差异有统计学意义(P<0.05)。结论HSP90α、lncRNA SNHG5及常规血清肿瘤标志物可用于辅助诊断早期CRC;相较于常规血清肿瘤标志物,HSP90α、lncRNA SNHG5联合诊断早期CRC价值更高,可为临床早期诊断CRC提供新的参考依据。

小分子热休克蛋白与肿瘤凋亡关系的研究进展

小分子热休克蛋白(small heat shock proteins,sHSPs)是众多热休克蛋白(heat shock proteins,HSPs)中的一大类,包括HSPB1、HSPB5、HSPB6、HSPB8等。近来研究表明,它们在许多信号通路扮演关键角色,这些信号通路与肿瘤的发生、抗放疗和凋亡的抑制有着许多联系,尤其是在肿瘤凋亡方面。本文对sHSPs在肿瘤凋亡途径方面予以综述。

小热休克蛋白HSP17.4与过氧化氢酶2互作调控其酶活性

【目的】为探究拟南芥小热休克蛋白HSP17.4与过氧化氢酶2的关系。【方法】构建带有组氨酸标签的小热休克蛋白HSP17.4的原核蛋白表达载体,将小热休克蛋白HSP17.4与过氧化氢酶2的重组蛋白诱导表达后进行体外免疫共沉淀试验,并利用过氧化氢酶活性试剂盒检测过氧化氢酶活力。【结果】成功构建了带有组氨酸标签的小热休克蛋白HSP17.4的蛋白表达载体,并通过体外免疫共沉淀试验发现带有组氨酸标签的小热休克蛋白HSP17.4能够将无纯化标签的过氧化氢酶2成功纯化出来,过氧化氢酶活性检测表明小热休克蛋白HSP17.4可以显著增强过氧化氢酶2活性。【结论】本研究证明小热休克蛋白HSP17.4与过氧化氢酶2存在相互作用,并且小热休克蛋白HSP17.4激活过氧化氢酶2酶活性,为进一步研究小热休克蛋白HSP17.4通过调控过氧化氢酶2参与非生物胁迫响应奠定基础。

大豆Hsp20基因家族生物信息学分析及高温高湿胁迫响应的分析

热激蛋白(Hsps)家族中的小热激蛋白(Hsp20)在保护植物免受非生物胁迫方面发挥至关重要的作用,为探究大豆Hsp20家族基因的特性及其对高温高湿胁迫的响应,对大豆进行了全基因组分析,本研究采用生物信息学方法对进化关系、保守结构域、染色体位置、启动子顺式调控元件和组织特异性表达情况进行预测分析,并采用同位素标记相对和绝对定量(iTRAQ)技术对湘豆3号和宁镇1号两个大豆品种在高温高湿胁迫下不同时间的蛋白表达量进行了分析。结果表明:在大豆基因组中共查找出33个GmHsp20基因,不均匀分布在16条染色体上并根据系统发育分析和亚细胞定位结果分为11个亚族。序列分析表明GmHsp20蛋白表现出较高的结构保守性,含有典型的ACD结构域,32个GmHsp20基因(96.96%)没有内含子,或只有1个内含子。启动子分析表明,GmHsp20基因含有大量与胁迫相关的顺式作用元件,其中MYB数目最多(110)个。基因组织特异性表达预测分析结果显示,除GmHSP22.6外,其余基因在各种组织和器官中均有表达。其中GmHSP18.5、GmHSP23.7、GmHSP15.2基因在所有组织中均高度表达。蛋白定量分析结果表明,与对照相比,宁镇1号和湘豆3号两个品种中,经高温高湿胁迫处理后,GmHSP18.5、GmHSP23.7、GmHSP26.0B、GmHSP17.8、GmHSP25.95个蛋白均上调表达,并且在两个品种间表达趋势基本一致,表明这些小热激蛋白家族成员可能参与了大豆对高温高湿胁迫的应答反应过程。本研究结果为进一步研究大豆小热激蛋白GmHsp20家族成员的功能提供有价值的信息。

肿瘤异常蛋白、热休克蛋白90α联合血清肿瘤标志物检测对非小细胞肺癌的诊断价值

目的 探讨肿瘤异常蛋白(TAP)、热休克蛋白90α(HSP90α)联合血清肿瘤标志物[神经元特异性烯醇化酶(NSE)、癌胚抗原(CEA)、细胞角质蛋白19片段抗原21-1(CYFRA21-1)]检测对非小细胞肺癌的诊断价值.方法 选取90例非小细胞肺癌患者和90例健康体检者,分别作为肺癌组和对照组,比较两组患者血清TAP面积及HSP90α、NSE、CEA、CYFRA21-1水平.以病理学检查结果为金标准,评估TAP面积、HSP90α、NSE、CEA、CY-FRA21-1联合检测对非小细胞肺癌的诊断价值.结果 肺癌组患者血清HSP90α、NSE、CEA、CYFRA21-1水平均明显高于对照组,TAP面积明显大于对照组,差异均有统计学意义(P﹤0.01).五项联合检测诊断非小细胞肺癌的灵敏度为93.33%,阴性预测值为91.55%,均高于血清CEA、NSE、CYFRA21-1、TAP面积、HSP90α单独检测.结论 TAP面积、HSP90α、NSE、CEA、CYFRA21-1联合检测可提高对非小细胞肺癌的诊断效能.

非小细胞肺癌患者热休克蛋白90β表达水平及其与病理学关系研究

目的探讨非小细胞肺癌(NSCLC)患者血浆热休克蛋白90β(Hsp90β)表达水平及其与病理学关系。方法选择2020年7月至2021年7月入住解放军海军陆战队医院的120例NSCLC患者作为患者组,另外选择同期80名在我院参与健康体检的健康者作为对照组。经标本收集、准备、样本制备、加样、温育、洗板、显色、终止、检测及计算等过程,采用上海信裕生物科技有限公司生产的酶联免疫分析仪对Hsp90β水平进行检测分析。另外给予患者组4个周期以上的顺铂+吉西他滨、顺铂进行化疗。比较患者组与对照组Hsp90β的阳性表达率;分析Hsp90β阳性表达率与病理学之间的关系;比较化疗治疗前后Hsp90β表达水平。结果①患者组Hsp90β阳性表达率为63.33%(76/120),显著高于对照组的18.75%(15/80),差异有统计学意义(P<0.05);②有淋巴结转移患者的Hsp90β阳性表达率显著高于无淋巴结转移患者(P<0.05),Ⅲ期患者的Hsp90β阳性表达率显著高于Ⅰ~Ⅱ期患者,差异有统计学意义(P<0.05);组织分化程度越高,患者Hsp90β阳性表达率越低,差异有统计学意义(P<0.05);③化疗后,NSCLC患者Hsp90β水平为(109.34±10.08)ng/ml,显著低于化疗前[(142.29±16.56)ng/ml],差异有统计学意义(P<0.05)。结论Hsp90β在NSCLC中的表达显著异常,且有无淋巴结转移、不同临床分期及组织分化者的表达差异显著,具有一定的临床检测意义。

玉米小分子热激蛋白ZmHSP17.7基因的克隆与功能分析

植物热激蛋白是一类代表性高温响应蛋白。以玉米种质POB21为材料,克隆了一个CDS序列长度为477 bp的小分子热激蛋白基因。该基因编码的蛋白含158个氨基酸,具有HSP20蛋白典型的ACD结构域,预测的等电点为5.36,分子量为17.746 k D,被命名为Zm HSP17.7。在水稻、拟南芥等植物基因组中都有其同源基因,进化和亚细胞定位分析表明,此基因属CI类小分子热激蛋白家族成员。Northern杂交分析表明,高温快速诱导Zm HSP17.7基因表达,15%PEG模拟干旱胁迫不诱导该基因表达,但在复合胁迫下干旱增强了高温的诱导效果。外源ABA也不影响该基因的表达。与野生型拟南芥相比,超表达Zm HSP17.7的转基因拟南芥在种子萌发和植株生长过程中表现出更强的高温和干旱耐受性,说明该基因可以在植物防御高温、干旱及复合胁迫中发挥一定作用。

番茄转ER-sHSP基因植株构建及其抗冷性研究

将CaMV35S启动子驱动的内质网小分子热激蛋白基因导入番茄,比较转基因、未转基因和转空载体番茄的抗冷能力。冷胁迫下,同对照相比,转基因番茄的冷害症状轻,叶绿素含量的损失少,体内积累的丙二醛(MDA)含量少,电解质外渗程度低,具有较高的净光合速率和最大光化学效率,并易于恢复由低温所引起的光抑制,表明转基因番茄具有较强的冷胁迫耐性,说明内质网小分子热激蛋白在植物抗冷过程中发挥重要作用。

小热休克蛋白MjHSP16.5对多肽纤维生长的抑制及对成熟纤维的解聚作用

包括老年痴呆症在内的许多疾病与蛋白质或多肽的淀粉样聚集(纤维化)有关.由于这类疾病的机制尚不清楚,因此还没有有效的预防和治疗手段.研究各种因素如小热休克蛋白对蛋白质或多肽淀粉样聚集的影响对开发防治相关疾病的药物具有重要意义.甲状腺素运载蛋白(TTR)及其突变体很容易形成淀粉样纤维,并与多种疾病相关.Mj HSP16.5是一种来源于嗜热古细菌Methanococcus jannaschii的小热休克蛋白,它在酸性条件下具有非常高的分子伴侣活性.本文研究了Mj HSP16.5对WTTR肽(在N端添加了色氨酸的TTR105-115片段,序列为WYTIAALLSPYS)纤维化的影响,发现Mj HSP16.5能够显著地抑制WTTR肽纤维的生长,且在Mj HSP16.5存在下,WTTR肽形成的纤维比正常条件下形成的要显著细小.尤其是Mj HSP16.5还可以使已经成熟的WTTR肽纤维解离.结果表明,Mj HSP16.5抑制多肽纤维的机理可能在于其能够与多肽纤维及纤维种子结合.

坛紫菜两种小分子热激蛋白(sHSP)基因的克隆及表达特征分析

小分子热激蛋白(s HSP)不仅在应激条件下高效表达,还在正常状态的细胞中广泛存在,参与一些重要细胞生理活动的调节。为研究坛紫菜应答高温和失水等逆境胁迫的分子机制,本研究以坛紫菜转录组测序获得的unigene序列为基础,采用RACE或直接PCR扩增,克隆获得了坛紫菜2种s HSP的全长基因:Ph Hsp22和Ph Dna J。序列分析结果表明,Ph Hsp22序列全长857 bp,包含一个519 bp的开放阅读框,所编码的多肽包含172个氨基酸,分子量为19.1 ku,等电点为5.24(收录号:KM102540);Ph Dna J序列全长1 616 bp,包含一个1 290 bp的开放阅读框,所编码的多肽包含429个氨基酸,分子量为46.1 ku,等电点为6.43,属于Hsp40亚家族(收录号:KM102541)。基因表达水平的定量分析结果表明,两个基因在高温胁迫不同时间水平和不同失水胁迫程度下的表达均呈现出一致的表达模式,即在胁迫初期表达水平显著上调,但随着胁迫的持续,这两个基因的表达水平开始逐渐下调。结果表明,这2个基因在逆境胁迫下的表达可能存在一个反馈调节机制。

家蚕HSP20·8基因体外表达及荧光原位杂交研究(英文)

前期研究发现,相对于其它组织器官,有一种低分子量热激蛋白在家蚕肾型卵中高量表达,并命名为低分子量热激蛋白HSP20.8。为了进一步阐明家蚕低分子量热激蛋白HSP20.8的基因结构、表达特性及其在家蚕染色体上的分布,根据HSP20.8基因cDNA序列设计特异引物,进行了克隆、表达及荧光原位杂交研究。结果表明,该基因含有1个561碱基对的开放阅读框(open reading frame,ORF),与cDNA序列比较分析发现该基因无内含子序列。重组蛋白的分子量在20 kD左右。热激蛋白基因HSP20.8在家蚕基因组中为单拷贝基因,其位点在染色体近中部区域。