Wilm′s tumor gene1肽疫苗Galinpepimut-S在肿瘤免疫治疗中的应用

目的为Wilm′s tumor gene1(WT1)肽疫苗Galinpepimut-S(GPS)用于肿瘤免疫治疗的后续研究提供参考。方法采用计算机检索中国知网、PubMed等数据库自建库起至2022年12月的肿瘤免疫治疗相关文献,总结GPS在肿瘤免疫治疗中的应用现状。结果GPS能激发自身免疫系统,对WT1抗原产生强烈免疫反应而发挥抗肿瘤作用,在卵巢癌、恶性胸膜间皮瘤、急性髓系白血病、多发性骨髓瘤的治疗中均显示出较好的疗效。结论以GPS为代表的肿瘤疫苗是未来肿瘤治疗的重要方向,需进一步进行临床研究,以获取更多数据。

Progress of CACNA1S Gene and Hypokalemic Periodic Paralysis

CACNA1 S gene is the gene encoding L-type calcium channel αa-subunit. CACNA1 S gene mutations can cause hypokalemic periodic pa- ralysis （HOKPP）. The related research speculated that CACNA1 S gene was the candidate genes which affect meat quality traits. In the present ar- ticle, the biological characteristics of CACNA1 S gene, structure, genetic diseases and the research development were respectively reviewed so as to provide a reference for further research.

Molecular Characteristics of S1 Gene of Infectious Bronchitis Virus Isolated from Chicken Proventriculus

Infectious bronchitis virus was isolated from swollen proventriculi of clinically ill chicken. The suspected virus samples (2/97, 3/97, 1/98) were adapted in SPF chicken embryos for virus isolation and identification. All the virus isolates were able to agglutinate chicken erythrocytes after treatment with trypsin, and interfer with the reproduction of Newcastle disease virus in chicken embryos, and have low antigenic relat-edness values with reference positive IBV. The isolates 2/97, 3/97, 1/98 RNAs extracted from the allantoic fluid of inoculated embryonated eggs were converted to cDNA by reverse transcription with 3'-primer of S1 gene of (IBV). Polymerase chain reaction (PCR) was performed with two primers which span the S1 gene. Amplified product of 1. 93 kb was subjected to EcoR I and BamH I digestion and the fragments obtained were the same as expected size. The PCR product was ligated to pBlueScript-SK ( + ) vector, and its nucleotide sequence was determined by the dideoxy-mediated chain termination method. Nucleotide sequence analysis showed 73. 6 - 99. 7% homology between the isolated IBV and the IBV strains in GenBank. The homology of amino acid was 71. 4 - 99.4%.

Prokaryotic Expression of Infectious Bronchitis Virus S1 Gene and Analysis of Biological Activity of Recombinant Protein

[Objective] To study the prokaryotic expression and antigenicity identification of S1 gene from avian infectious bronchitis virus （IBV）. [Method] The S1 gene was cloned into a pMD18-T vector to yield a recombinant plasmids pMD18-T-IBV-S1. Then S1 gene was inserted into the multiple cloning site of a prokaryotic expression vector pET-32a （ ＋ ）. The recombinant plasmid was transformed into E. coil BL21. The recombinant protein was induced by IPTG and measured by SDS-PAGE and western-blotting. [Result] The S1 gene was successfully expressed in E. coil BL21, the fusion proteins were about 66.0 kDa in a form of inclusion body. Western-blotting test showed that the recombinant proteins could be identified by IBV polyclonal antibody. [ Conclusion] The recombinant proteins of S1 gene have the antigenicity, which lays a good foundation for further research on new generation vaccine of IBV.

谷胱甘肽S转移酶P1和X线修复交错互补基因1基因多态性与前列腺癌化疗敏感性及预后关系研究

目的:探究前列腺癌患者谷胱甘肽S转移酶P1(GSTP1)和X线修复交错互补基因1(XRCC1)基因多态性与化疗敏感性及预后的关系。方法:选取2018年5月至2021年5月行雄激素剥夺治疗+双药化疗的前列腺癌患者103例,收集患者临床资料,采用PCR-PFLP方法对患者行基因分型,并分析其GSTP1-rs1695位点和XRCC1-rs25487位点的多态性,分析其与化疗敏感性的关系,并探究GSTP1和XRCC1基因多态性与患者3年生存率的相关性。结果:103例前列腺癌化疗患者GSTP1-rs1695位点和XRCC1-rs25487位点分布均符合Hardy-Weinberg平衡(χ2=9.794,P>0.05)。GSTP1-rs1695位点中AA基因型占比为65.05%(67/103),AG基因型占比为23.30%(24/103),GG基因型占比为11.65%(12/103);XRCC1-rs25487位点中AA基因型占比为29.13%(30/103),AG基因型占比为50.49%(52/103),GG基因型占比为20.39%(21/103)。GSTP1-rs1695 AA型化疗敏感性为35.82%,低于AG/GG型58.33%(P<0.05)。XRCC1-rs25487 AA型化疗敏感性为40.00%,AG/GG型45.21%,两者差异无统计学意义(P>0.05)。GSTP1-rs1695、XRCC1-rs25487不同表型患者3年无进展生存率之间无明显差异(P>0.05)。GSTP1-rs1695 AA型3年总生存率低于AG/GG型;XRCC1-rs25487 AA型低于AG/GG型(P<0.05)。多因素COX回归分析结果显示,GSTP1-rs1695 AA型、XRCC1-rs25487 AA型均为前列腺癌患者化疗后3年总生存期的独立影响因素。结论:GSTP1-rs1695、XRCC1-rs25487基因多态性对前列腺癌患者化疗敏感性和预后均有一定影响,GSTP1-rs1695和XRCC1-rs25487 A等位基因突变均可导致更短的3年生存率,G等位基因突变可带来更好的化疗敏感性和生存期。

Expression of GST-IL-1 fusion gene

Two GST-IL-1 fusion genes were constructed by inserting different cDNA fragments of human interleukin1 (IL-1) into the 3'-terminus of GST gene in the fusion protein expression vector pGEX-4T. After IPTG induction ,SDS-PAGE was employed to detect the gene expression. No corresponding protein encoded by GST gene fused with the whole-length 816 bp IL-1 cDNA was observed, nor was free GST protein. However, the fusion protein of GST and IL-1 cDNA without the 189 bp at the 5'- terminus was detected, amounting to 30% of the total bacterial protein expressed. This might suggest that the sequence of 1-189 bp of IL-1 cDNA affected the expression of the fusion gene. That is to say, the downstream sequence distant from the translation start codon AUG in the target gene could significantly affect the expression of the fusion gene.

传染性支气管炎病毒类M_(41)地方分离株S_1基因克隆及高变区序列分析

传染性支气管炎病毒（ＩＢＶ）分离株ＱＤ经ＲＴ－ＰＣＲ扩增出约１．７ｋｂＳ１糖蛋白基因ｃＤＮＡ，修饰后插入ｐＵＣ１８ＳｍａｌⅠ／ＥｃｏＲＩ位点构成质粒ｐＵＣＱＤＳ１。对克隆的Ｓ１基因５′端高变区序列测定显示，起始密码上游６０碱基和下游３８０碱基中与参考株Ｍ４１Ｓ１基因序列仅有１个碱基的差异，表明ＱＤ为一类Ｍ４１分离株。

传染性支气管炎病毒S_1基因DNA免疫质粒的构建及其免疫原性

为探讨ＤＮＡ免疫防制传染性支气管炎（ＩＢ）的可能性，以克隆的Ｍａｓｓｃｈｕｓｅｔｅ型类Ｍ４１地方分离ＱＤ株Ｓ１基因为免疫原基因，引入终止密码后插入ＳＶ４０启动子、增强子下游和ＳＶ４０ｐｏｌｙＡ信号上游，构建了Ｓ１基因ＤＮＡ免疫表达质粒ｐＳＶＱＤＳ１。将大量扩增并经聚乙二醇纯化的ｐＳＶＱＤＳ１溶于ＰＢＳ，以３００μｇ／只的剂量肌肉注射免疫小鼠，于４周后采集分离免疫小鼠血清进行鸡胚病毒中和试验。结果表明，ｐＳＶＱＤＳ１能够诱导产生针对传染性支气管炎病毒（ＩＢＶ）Ｍ４１株的中和抗体，具有良好的免疫原性。

PDRG1 at the interface between intermediary metabolism and oncogenesis

PDRG1 is a small oncogenic protein of 133 residues. In normal human tissues, the p53 and DNA damageregulated gene 1(PDRG1) gene exhibits maximal expression in the testis and minimal levels in the liver. Increased expression has been detected in several tumor cells and in response to genotoxic stress. High-throughput studies identified the PDRG1 protein in a variety of macromolecular complexes involved in processes that are altered in cancer cells. For example, this oncogene has been found as part of the RNA polymerase Ⅱ complex, the splicing machinery and nutrient sensing machinery, although its role in these complexes remains unclear. More recently, the PDRG1 protein was found as an interaction target for the catalytic subunits of methionine adenosyltransferases. These enzymes synthesize S-adenosylmethionine, the methyl donor for, among others, epigenetic methylations that occur on the DNA and histones. In fact, downregulation of S-adenosylmethionine synthesis is the first functional effect directly ascribed to PDRG1. The existence of global DNA hypomethylation, together with increased PDRG1 expression, in many tumor cells highlights the importance of this interaction as one of the putative underlying causes for cell transformation. Here, we will review the accumulated knowledge on this oncogene, emphasizing the numerous aspects that remain to be explored.

Oxidative stress regulated heme-oxygenase-1 and glutathione S-transferase-m1 gene expression changes in cell lines exposed to melanins

To investigate the effects of oxidative stress on substantia nigra neuronal degeneration and death in patients with Parkinson＇s disease, we treated neuroblastoma cells （SK-N-SH） and glioma cells with Fenton＇s reagent, iron chelating agent, neuromelanin and dopamine melanin. We investigated the changes in expression of nine oxidative stress-related genes and proteins. The levels of mRNAs for heme-oxygenase-1 and glutathione S-transferase-ml were significantly reduced in SK-N-SH cells exposed to oxidative stress, and increased in glial cells treated with deferoxamine. These results revealed that SK-N-SH neurons react sensitively to oxidative stress, which implies different outcomes between these two types of cells in the substantia nigra. Moreover, the influences of neuromelanin and dopamine melanin on cell function are varied, and dopamine melanin is not a good model for neuromelanin.

人肺癌GSTM1基因多态性与p53突变的相关性

目的 探讨谷胱苷肽 S转移酶 μ1(GSTM1)基因的多态性与抑癌基因 p5 3突变在人肺癌发生中的关系。方法 收集 4 8例人肺癌标本 ,HE染色做病理诊断 ,抽提基因组 DNA,PCR扩增 GSTM1基因的第 4外显子 ,聚丙烯酰胺凝胶电泳分析基因的多态性。对相应的肺癌标本用免疫组织化学的方法做突变型 P5 3蛋白表达的检测 ,分析二者的相关性。结果 在人的肺癌组织中 ,GSTM1基因的缺失率较高 ,达 5 4 .2 % ;突变型 P5 3蛋白总的表达率为 5 6 .3% ,其中GSTM1基因缺失者与非缺失者的 p5 3突变率分别为 73.1%和 36 .4 % ,二者之间有显著性差异 ,P<0 .0 5。结论 在人肺癌组织中 ,GSTM1基因的多态性与 p5 3基因突变明显相关 ,GSTM1基因的缺失可能会导致 p5

百日咳杆菌毒素S_1亚单位与谷胱甘肽S-转移酶融合基因在大肠杆菌中表达及其一步纯化

研究了百日咳杆菌毒素Ｓ１亚单位与谷胱甘肽Ｓ－转移酶融合蛋白（ＧＳＴ－Ｓ１）在大肠杆菌（Ｅ．ｃｏｌｉ）中的表达，并一步纯化了重组ＧＳＴ－Ｓ１。首先用聚合酶链反应（ＰＣＲ）扩增出长度为５６０ｂｐ的编码百日咳毒素Ｓ１亚单位的ＤＮＡ片段。该片段比原编码Ｓ１蛋白的ＤＮＡ片段在其３′端缺失了１３８个碱基，将其按正确的阅读框克隆入质粒ｐＧＥＸ中ＧＳＴ基因的３′端，构成ＧＳＴ－Ｓ１融合基因表达载体ｐＧＥＸ－Ｓ１。经异丙基硫代－β－Ｄ－半乳糖苷（ＩＰＴＧ）诱导表达和十二烷基磺酸钠－聚丙烯酰胺凝胶电泳（ＳＤＳ－ＰＡＧＥ），可见所表达的ＧＳＴ－Ｓ１融合蛋白存在于细菌上清，为可溶性蛋白。分子量为４９ｋｕ处有明显的蛋白表达带。用谷胱甘肽（ＧＳＨ）亲和层析系统，一步纯化出ＧＳＴ－Ｓ１融合蛋白。最后经凝血酶的消化，得到２３ｋｕ的重组百日咳杆菌毒素Ｓ１亚单位蛋白。

鸡传染性支气管炎北京地方株S_1基因的克隆与鉴定

利用反转录套式聚合酶链反应（ＲＴｎｅｓｔｅｄＰＣＲ）技术从北京地区３株鸡传染性支气管炎病毒（ＩＢＶ）分离株（ＢＪ１，ＢＪ２，ＢＪ３）中扩增出１０５４ｂｐＳ１基因高变区。利用限制性内切酶ＳｉｎⅠ和ＰｓｔⅠ的酶切位点分析图谱进一步证实了ＲＴｎｅｓｔｅｄＰＣＲ的特异性。将３段Ｓ１基因分别克隆到ｐＵＣ１９质粒中，获得重组质粒ｐＵＣＩＢＶＳ１ＢＪ１，ｐＵＣＩＢＶＳ１ＢＪ２和ｐＵＣＩＢＶＳ１ＢＪ３。

焦炉工血清GST活力与尿1-羟基芘和GSTM1、GSTT1基因多态的关系

目的研究血清谷胱甘肽硫转移酶(GST)能否作为焦炉工人多环芳烃的暴露评价指标,同时探讨GSTM1、GSTT1基因多态性与血清GST活力的关系。方法选择某焦化厂39名男性焦炉工人和44名男性对照工人,采用统一的调查表调查一般情况。采集静脉血分析血清GST活力和GSTM1、GSTT1基因型,采集尿样分析尿1-羟基芘(1-OHP)浓度。血清GST活力用试剂盒检测;尿1-羟基芘(1-OHP)浓度作为多环芳烃内暴露剂量,用碱水解-高效液相色谱方法测定;GSTM1和GSTT1基因多态性分析采用PCR方法。结果焦炉工人尿1-OHP浓度(中位数为5.60μmol/mol肌酐)和血清GST活力(中位数25.75U/ml)分别高于对照组(尿1-OHP浓度:中位数1.32μmol/mol肌酐,血清GST活力:14.54U/ml),差异均有统计学意义(均P<0.001)。GSTM1(-/-)和GSTT1(-/-)型工人的血清GST活力分别与GSTM1(-/+,+/+)和GSTT1(-/+,+/+)型工人的血清GST活力相比,差异均无统计学意义(均P>0.05)。广义线性回归分析显示,尿1-OHP对血清GST的影响具有统计学意义(P<0.01)。血清GST活力和尿1-OHP浓度存在统计学正相关(r=0.357,P<0.001,n=83)。结论焦炉工人血清GST有可能作为多环芳烃暴露评价的参数;未见GSTM1和GSTT1基因缺失对血清GST活力的影响。

传染性支气管炎病毒S_1基因遗传变异研究

本文利用计算机互联网分析了传染性支气管炎病毒 ( IBV) Buead株 (呼吸型 )和 Z株(肾病型 ) S1基因的遗传变异规律。经与 Genbank中 50余个传染性支气管炎病毒的 S1基因序列比较研究表明 :Beaud株和 Z株均存在着高度变异和相对保守区 ,两株病毒 S1基因含有 5～ 6个插入变异区。本文同时分析了两株病毒 S1蛋白氨基酸序列的变异规律 ,研究表明 :各株传染性支气管病毒之间 S1蛋白的氨基酸序列有局部变异 ,其中 1 0 5～ 1 0 6个氨基酸保持恒定不变。功能位点分析表明 :Z株与 Buead株抗原位点的位置和组成已发生变异 ,糖基化位点除 Z株出现两个新位点外 ,其位置没有发生变化 。

禽传染性支气管炎病毒S_1基因玉米表达载体的构建

禽传染性支气管炎病毒主要编码3种结构蛋白,其中S蛋白的S1蛋白是宿主的主要保护性抗原,能诱导机体产生中和抗体和血凝抑制抗体,并与病毒的组织嗜有关。本研究选取具有代表性的禽传染性支气管炎病毒分离株SAIB14和SAIB4,以其S1基因克隆质粒pUCSAIB14和pUCSAIB4为模板,用具有高保真度的pfu酶分别扩增,得到含先导序列的S1基因片段。把扩增产物分别通过ClaI和BamHI酶切纯化,替换中间载体pUGFPocs的GFPm1基因,构建中间表达载体pUSAIB14和pUSAIB4。用KpnI和HindIII双酶切重组质粒pUSAIB14和pUSAIB4,回收Ubi-S1-Tocs片段,定向插入到pCAMBIA1300载体的多克隆位点。经酶切和PCR鉴定,证明获得了S1基因的玉米表达载体pCUSAIB14和pCUSAIB4。外源基因导入受体植物能否有效表达,表达载体构建是关键因素,构建时选用表达载体的类型、启动子和终止子、目的基因插入位点等都有影响。本研究用BamHI和ClaI双酶切载体pUGFPocs,用S1基因扩增片段替换GFPm1基因,将S1基因置于Ubi启动子和T-ocs终止子的控制之下,有助于S1蛋白的高效表达,最后将Ubi-S1-Tocs单元HindIII和KpnI双酶切下来,插入到pCAMBIA1300的多克隆位点,得到可用于农杆菌介导的转化或直接转化的植物表达载体pCUSAIB4和pCUSAIB14。Ubi启动子来自玉米,属组成型启动子,?

Alzheimer病患者APP及PS1基因的表达水平

为了检测Alzheimer病(Alzheimer’s disease,AD)患者外周血中淀粉样前体蛋白(Amyloid Precursor Protein,APP)基因及早老素1(Presenilin 1,PS1)基因的表达情况,进而探讨APP及PS1基因的表达与AD的相关性,采用SYBRGreenⅠ的方法对45例AD患者、25例血管性痴呆(vascular dementia,VD)患者及60名正常对照组样本的mRNA进行绝对定量,检测得到APP基因及PS1基因在对照组中的表达水平分别为0.026±0.005 amol/μg cDNA和0.026±0.004 amol/μg cDNA;在AD患者组中的表达量分别为0.044±0.006 amol/μg cDNA和0.051±0.011amol/μg cDNA;,在VD患者组中的表达水平分别为0.072±0.013 amol/μg cDNA和0.039±0.005 amol/μg cDNA。经显著性检验,AD患者组APP基因的表达水平上调,t=2.639,P<0.01;PS1基因的表达水平同样呈上调趋势,t=2.173,P<0.05,差异均具有统计学意义。VD患者组APP基因的表达水平上调,t=3.028,P<0.01;PS1基因的表达水平也同样呈上调趋势,t=2.012,P<0.05,均有显著性差异。因此,APP及PS1基因的表达水平的增高并不一定与AD发生特异性关联,而可能与多种导致痴呆的脑部病变发生关联。

功能性消化不良患者血浆中NPSR1、CGRP及IL-6的表达水平及临床意义

目的探讨功能性消化不良(functional dyspepsia,FD)患者血浆中神经肽S受体1(neuropeptide S receptor 1,NPSR1)、降钙素基因相关肽(calcitonin gene related peptide,CGRP)及白介素-6(interleukin-6,IL-6)的表达水平及其临床意义。方法选取2012年4月至2015年10月就诊于本院的143例FD患者纳入FD组,其中,上腹痛综合征(epigastric pain syndrome,EPS)70例(EPS组),餐后不适综合征(postprandial distress syndrome,PDS)73例(PDS组)。选取同期于本院体检的健康者80例纳入对照组,采用酶联免疫吸附测定(ELISA)检测所有研究对象血浆中NPSR1、CGRP及IL-6的表达水平,并进行统计学分析。结果 FD组患者最主要的临床症状为消化不良或胀气(82.52%),其次为嗳气(79.72%)、疲乏(76.22%)及腹痛(75.52%)。FD组患者血浆中NPSR1、CGRP、IL-6的表达水平分别为(170.25±16.40)、(117.43±15.58)、(92.75±6.80)pg/ml,对照组分别为(207.10±14.42)、(172.55±8.90)、(65.60±7.35)pg/ml,两组比较差异具有显著性(P<0.05)。PDS组患者血浆中NPSR1、CGRP、IL-6水平分别为(158.55±17.43)、(106.72±14.65)、(88.42±7.15)pg/ml,EPS组分别为(182.00±16.66)、(128.54±16.64)、(97.50±6.75)pg/ml,两组比较差异显著(P<0.05)。结论FD患者血浆中NPSR1、CGRP表达水平下降,而IL-6表达水平升高,提示NPSR1、CGRP及IL-6的表达水平与FD的发生密切相关。

MDR1、GSTπ特异性siRNA真核表达载体的构建及表达

目的构建多药耐药基因(MDR1)、谷胱甘肽S-转移酶(GSTπ)特异性小干扰RNA(siRNA)真核表达载体并检测其表达。方法参照siRNA模板设计原则,设计并化学合成2条siRNA模板序列,退火后将其插入质粒pSilencer2.1-U6,限制性酶切和基因测序进行鉴定。脂质体介导下转染K562/Adr细胞,实时荧光定量PCR分析MDR1、GSTπmRNA的表达,荧光免疫组化检测Pgp、GSTπ蛋白的表达。结果重组质粒pSilenc-er2.1-MDR1、GSTπ经酶切、测序分析表明siRNA模板序列成功插入预计位点,并且序列正确。用pSilencer-mdr1、pSilencer2.1-GSTπ分别转染K562/Adr细胞株,mdr1mRNA表达量下降了71.5%,GSTπmRNA表达量下降了39.8%,荧光免疫组化显示Pgp、GSTπ表达均显著减少(P<0.01)。结论成功构建了MDR1、GSTπ特异性siRNA真核表达载体,该载体可不同程度逆转K562/Adr细胞的多药耐药。

GSTP1、MTHFR基因多态性与PF方案治疗食管癌疗效相关性研究

目的：了解食管癌患者谷胱甘肽S转移酶P1（glutathione S-transferase Pi-1,GSTP1）,亚甲基四氢叶酸还原酶（methylenetetrahydrofolate reductase,MTHFR）基因多态性分布频率,探讨GSTP1、MTHFR基因多态性与食管癌患者PF方案（顺铂联合5-氟尿嘧啶）化疗疗效相关性。方法：从168例接受PF方案化疗的食管癌病例中采外周血提取DNA,采用PCR法扩增目的基因片段,直接测序法分析GSTP1、MTHFR基因多态性,每两周期化疗后评价疗效一次,按照实体瘤的疗效评价标准进行评价。结果：168例食管癌患者PF方案化疗疗效评价（实体瘤的疗效评价标准RECIST 3.0）,CR 19例（11.3%）,PR 60例（35.7%）,SD 48例（28.6%）,PD 41例（24.4）,食管癌患者GSTP1基因野生型（AA）有效率为22.0%,杂合型（AG）＋纯合型（GG）有效率为25.0%,MTHFR C667T基因野生型（CC）有效率为14.3%,杂合型（CT）＋纯合型（TT）有效率为32.7%,MTHFR A1298C基因野生型（AA）有效率为17.3%,杂合型（AC）＋纯合型（CC）有效率为29.8%,其中GSTP1基因野生型（AA）与杂合型（AG）＋纯合型（GG）的OR=2.520,95%CI：11.237-25.191,P=0.012,MTHFR C6 6 7 T基因野生型（CC）与杂合型（CT）＋纯合型（TT）的OR=1.933,95%CI：5.987-16.354,P=0.032,MTHFR A1298C基因野生型（AA）与杂合型（AC）＋纯合型（CC）的OR=3.514,95%CI：19.018-27.332,P=0.511。结果显示食管癌患者GSTP1基因及MTHFR C667T基因多态性与PF方案化疗后疗效相关,且杂合型及纯合型疗效优于野生型。结论：GSTP1及MTHFR-C677T基因多态性与5-氟尿嘧啶的疗效具有相关性,而MTHFR-A1298C基因多态性与5-氟尿嘧啶的疗效无明显相关性,故检测GSTP1及MTHFR-C677T基因多态性可预测PF方案化疗疗效。