Gene X-pert MTB/RIF检测对肺结核病的诊断价值研究

目的 研究分析肺结核病应用Gene X-pert MTB/RIF检测的诊断价值。方法 选取2022年3—10月在本院就诊的疑似肺结核病患者164例为研究对象,所有患者均给予结核分枝杆菌培养检查、痰涂片抗酸染色法诊断、Gene X-pert MTB/RIF检测,以结核分枝杆菌培养检查结果为金标准,比较痰涂片抗酸染色法诊断与Gene X-pert MTB/RIF检测的阳性率以及诊断准确性、灵敏度、特异度。结果 痰涂片抗酸染色法诊断阳性率为21.34%(35/164),Gene X-pert MTB/RIF检测阳性率为35.98%(59/164),Gene X-pert MTB/RIF检测明显高于痰涂片抗酸染色法诊断(P<0.05)。痰涂片抗酸染色法诊断的准确性为85.37%,灵敏度为59.65%,Gene X-pert MTB/RIF检测的准确性为95.12%,灵敏度为94.74%,Gene X-pert MTB/RIF检测明显高于痰涂片抗酸染色法诊断(P<0.05)。结论 在肺结核病诊断中,Gene X-pert MTB/RIF检测的阳性率更高,同时诊断准确率与灵敏度也更高,为肺结核病的诊断与治疗提供了可靠的指导依据。

肺泡灌洗液Gene X-pert MTB/RIF在肺结核诊断中的应用价值

目的探讨支气管肺泡灌洗液Gene X-pert MTB/RIF(简称X-pert)检查对成年人肺结核的诊断价值。方法收集2019年10月至2020年7月湖北省十堰市太和医院165例高度疑似肺结核患者的肺泡灌洗液,完善X-pert检查及BALF涂片检测,分别以病原学诊断和临床诊断为诊断金标准,分析X-pert诊断结核的阳性率,评估X-pert对BALF涂片阴性肺结核的诊断价值,并分析X-pert在成人肺结核中的诊断准确性。结果最终诊断结核81例,X-pert诊断结核阳性率为39.39%(65/165),BALF涂片的阳性率22.42%(37/165),X-pert诊断结核的阳性率明显高于BALF涂片,差异有统计学意义(P<0.05);在81例结核病例中,X-pert真阳性率为77.78%(63/81),分别以病原学诊断和临床诊断为诊断金标准,X-pert在病原学诊断结核中阳性率为82.00%(41/50),敏感度为82.00%,特异度为79.13%。在临床诊断结核中阳性率为70.97%(22/31),敏感度为70.97%,特异度为67.91%。在非结核组出现X-pert阳性2例,假阳性率为2.38%(2/84);以BALF涂片为金标准,在44例BALF涂片阴性的疑似病例中,X-pert检测出结核分枝杆菌阳性27例,检出率为61.36%(27/44)。结论支气管肺泡灌洗液Gene X-pert MTB/RIF在结核诊断中敏感性高,且在BALF涂片阴性时可快速检测出结核分枝杆菌,具有较高的临床实用价值。

Gene X-pert MTB/RIF检测对肺结核病诊断的价值

目的探讨Gene X-pert MTB/RIF检测对肺结核病诊断的价值。方法选取2020年5月—2021年10月期间在张家港市第一人民医院接受治疗的拟诊断为肺结核病患者113例为研究对象,所有患者均接受Gene Xpert MTB/RIF系统分子检测、结核分枝杆菌(MTB)培养和抗酸染色镜检诊断,以Gene X-pert MTB/RIF系统分子检测结果为观察组,以MTB培养检测结果为对照1组,以痰涂片抗酸染色镜检诊断结果为对照2组。对比3组诊断结果。结果结核病患者诊断结果中,以对照1组MTB培养检测结果为金标准,检测阳性39例(34.51%),观察组诊断阳性率(35.40%)高于对照2组(21.24%),差异有统计学意义(χ^(2)=12.250,P<0.05)。观察组诊断结果准确度、灵敏度高于对照2组,差异有统计学意义(P<0.05)。结论在对肺结核病诊断的诊断中,Gene X-pert MTB/RIF检测阳性率显著高于抗酸染色镜检诊断。

Gene X-pert Mtb/RIF检测技术与抗酸染色和BD960培养、药敏的比对研究

目的：评价Gene X-pert Mtb/RIF检测痰标本诊断结核病和结核菌对利福平耐药的效能。方法：采用2014年10月-2015年7月太原市第四人民医院收集的确诊结核病患者的痰标本进行涂片、BD960培养、BD960药敏试验及Gene Xpert Mtb/RIF检测,应用统计学方法对Gene Xpert Mtb/RIF与不同检测方法进行敏感度分析。结果：Gene X-pert Mtb/RIF检测技术敏感度均高于涂片和BD960培养（P〈0.05）,利福平耐药与BD960利福平耐药无统计学差异（P〉0.05）。结论：Gene Xpert Mtb/RIF检测技术是一种快速、自动化程度高、操作简便的结核病分子生物学诊断技术,为临床快速诊断结核病及是否对利福平耐药提供了有力的实验室佐证。

DNA repair gene XRCC1 polymorphisms and susceptibility to childhood acute lymphoblastic leukemia: a meta-analysis

Objective： To estimate the relationship between genetic polymorphisms of X-ray repair cross- complementing group 1 （XRCC1） and the susceptibility to childhood acute lymphoblastic leukemia （ALL）. Methods： Relevant case-control studies were enrolled in the meta-analysis. We applied Rev Man 4.2 software to pool raw data and test studies＇ heterogeneity and to calculate the incorporated odds ratio （OR） and 95% confidence interval （95% CI）. Results： Our data showed that the OR for the Gln allele of the Arg399Gln polymorphism, compared with the Arg allele, was 1.35 （95% CI, 1.16-1.57; P〈0.0001） for childhood ALL patients. Similarly, the homozygous genotype Gln/Gln and heterozygous genotype Arg/Gln both significantly increased the risk of childhood ALL compared with the wild genotype Arg/Arg （OR =1.58; 95% CI, 1.13-2.21; P=0.008; OR =1.51; 95% CI, 1.21-1.87; P=0.0002）. The dominant model of Arg399Gln was associated with childhood ALL risk （OR =1.54; 95% CI, 1.25-1.89; P〈0.0001）. The ethnic subgroup analysis demonstrated that the Gln allele in all five ethnic groups was prone to be a risk factor for childhood ALL just with different degrees of correlation while Arg194Trp SNP showed a protective or risk factor or irrelevant thing in different races. Conclusions： XRCC1 399 polymorphism may increase the risk of childhood ALL. Different ethnic groups with some gene polymorphism have different disease risks.

失活X染色体基因逃逸与系统性红斑狼疮的性别二态性

X染色体失活可平衡女性中两条X染色体的基因剂量。越来越多的证据表明,失活X染色体上存在许多能够逃逸失活的基因。逃逸的机制涉及到DNA、RNA、组蛋白的表观修饰以及众多的调控蛋白和染色质的空间结构。失活X染色体基因逃逸的研究为人类疾病(特别是自身免疫性疾病)性别二态性的研究开辟了新的途径。目前已证实包括TLR7、CD40L、IRAK-1、CXCR3、CXorf21等失活X染色体基因逃逸是系统性红斑狼疮(systemic lupus erythematosus,SLE)女性好发的重要原因。本文主要综述了失活X染色体上基因逃逸以及与SLE性别二态性形成的分子机制。阐明SLE性别二态性形成的分子机制,不仅对疾病的诊断、治疗具有重要意义,而且对深入揭示人类免疫系统的发育及调控机理也有重要的理论意义。

伴有癫痫的脆性X综合征家系1例

脆性X综合征(fragile X syndrome,FXS)是FMR1基因CGG异常重复扩增导致的疾病。本文报告1对经基因检测诊断为FXS的兄弟,2例患者分别为15岁和14岁,均存在语言障碍、智力障碍、注意力缺陷障碍、孤独症谱系障碍和FXS特征性面容等临床表现,其中先证者伴有罕见的晚发性癫痫发作,经左乙拉西坦治疗效果良好,而其弟弟经反复随访未见脑电图异常。该对病例提示FXS临床表型具有多样性和异质性。

IL-2RG基因c.675 C>A突变引起X-连锁重症联合免疫缺陷病患儿的基因检测及实验室与临床结果分析

目的探讨白细胞介素-2受体共同r链(interleukin 2 receptor gamma,IL-2RG)基因新发变异导致患儿重症联合免疫缺陷病(severe combined immunodeficiency,SCID)的分子遗传学特点和临床特征。方法分析西北妇女儿童医院儿童血液内科收治的一例重症联合免疫缺陷病患儿的临床资料、实验室结果及基因检测数据。结果一例两个月男婴,出生后反复感染入院治疗,患儿血细胞检测结果提示白细胞总数正常,但淋巴细胞明显减少;淋巴细胞亚群结果显示总T(CD3+),辅助T(CD3+CD4+),杀伤T(CD3+CD8+)和NK(CD3-CD16+CD56+)淋巴细胞占比明显减低,而B(CD3-CD19+)淋巴细胞占比明显升高;IgG明显减低,IgM和IgA小于检测下限;该患儿在感染状态下细胞因子水平未明显升高。患儿母亲家系中近3代有9例男性在出生后1岁内因反复感染致死,核心家系全外显子组测序结果发现,患儿X染色体IL-2RG基因(chrX:70329160)存在半合新发错义突变[c.675 C>A,p.S225R(p.Ser225Arg)],其母亲为携带者。依据以上证据患儿被确诊为X连锁重症联合免疫缺陷病(X-SCID)。随后每月静脉注射免疫球蛋白并服用常规抗生素和抗病毒药物预防感染,为患者造血干细胞移植做准备。因患儿出生后已接种卡介苗,患儿6月龄出现了播散性卡介苗病。经治疗后行造血干细胞移植。结论X-SCID患儿机体免疫功能缺陷严重,危及生命,接种活疫苗可能导致严重感染;该研究发现IL-2RG基因c.675 C>A突变是先证者X-SCID遗传学病因的新发致病变异,扩充了X-SCID致病基因IL-2RG的基因变异谱。

脆性X综合征遗传学诊断方法研究进展

脆性X综合征(FXS)是导致智力障碍和发育障碍的主要单基因病之一,呈X连锁不完全显性遗传。FXS的病因是FMR1基因内(CGG)n重复序列的不稳定扩展及其上游CpG岛的异常甲基化,进而导致脆性X智力低下蛋白(FMRP)减少或缺乏,FMRP的水平直接关系到临床表型的严重程度。临床表现和基因检测是诊断FXS的主要依据。然而,FMR1基因分子结构和遗传模式的特殊性使得FXS的分子诊断和遗传咨询面临挑战。因此,如何简便而准确地进行FMR1基因检测一直是临床关注的焦点。文章针对FXS遗传学诊断方法的研究进展进行综述,旨在促进FXS的规范诊断,为临床提供帮助。

HBV-HCC中HBx与免疫微环境的交互作用

乙型肝炎病毒X蛋白(HBx)是乙型肝炎病毒X基因(HBX)将自身DNA整合至人基因组,进而合成的多功能蛋白。HBX基因的表达受肝细胞免疫、微环境和机体免疫的监视和调控,其表达的蛋白也可通过激活肝星状细胞、参与机体免疫调节、调控炎性细胞因子和诱导细胞外基质重塑等参与肝细胞癌(HCC)抑制性免疫微环境的形成。HBx与免疫微环境的相互作用是影响乙肝病毒相关肝细胞癌(HBV-HCC)发生、发展的主要因素之一。深入研究HBx与免疫微环境相互作用机制,探索促进HBV-HCC抑制性免疫微环境形成的机制,有助于开发新型抗HCC药物,改善患者预后。本文就HBx与HBV-HCC免疫微环境的研究进展进行综述。

策勒黑羊X染色体多胎性状的关联分析

为促进多胎性状策勒黑羊品种的培育,以策勒黑羊多胎性状和X染色体分子标记为对象,探究策勒黑羊多胎性状在X染色体上的遗传解析。选择100只策勒黑羊进行基因分型,利用PLINKv1.90进行质量控制,同时对X染色体上的SNP位点和策勒黑羊的多胎性状进行关联分析,选取P<0.01的SNP位点进行标记,将筛选出的SNP位点附近的基因进行注释和分析,获得X染色体多胎性的候选基因。结果表明,有14个SNPs与策勒黑羊X染色体多胎性状在全基因组范围内显著相关。共筛选出20个候选基因,对20个候选基因进行生物学功能分析,多胎性状相关联的候选基因6个,其中,FTH1基因已有文献报道是多胎性状的候选基因。

HUWE1基因突变合并KDM5C基因突变导致X连锁的智力障碍1例

报道1例HUWE1基因突变合并KDM5C基因突变导致X连锁的智力障碍患者的临床资料,并进行文献复习。

TGF-β2和geneX对BrdU标记骨髓间充质干细胞增殖与成骨分化的作用

目的研究TGF-β2和gene X对Brd U标记的骨髓间充质干细胞增殖与成骨分化作用的影响.方法采用全骨髓贴壁培养法分离骨髓间充质干细胞,传代并鉴定,设实验组和空白对照组,实验组分4组:A组:Brd U标记后的BMSCs组;B组:Brd U标记后的BMSCs+TGF-β2组;C组:Brd U标记后的BMSCs+gene X组;D组:Brd U标记后的BMSCs+gene X+TGF-β2组.空白对照组为Brd U标记后的单纯BMSCs加入基础培养基避光培养.诱导培养后观察骨髓间充质干细胞生长形态、检测生长动力学(methyl thiazolyl tetrazolium,MTT)、碱性磷酸酶(ALP)和钙定量、进行细胞Von-Kossa法染色,观察成骨分化作用.结果 (1)4组BMSCs吸光度值(OD)分析比较显示:细胞组间差异有统计学意义(P<0.05);(2)各组BMSCs成骨诱导后碱性磷酸酶(ALP)和钙定量检测结果显示:细胞组间差异有统计学意义(P<0.05);(3)进行细胞Von-Kossa法染色,D组可见大量钙结节;C组可见较多钙结节;B组可见部分钙结节;A组可见少量钙结节;空白对照组未见钙结节.结论 (1)TGF-β2可促进骨髓间充质干细胞的增殖和诱导其向成骨细胞分化;(2)gene X可促进骨髓间充质干细胞向成骨细胞分化,且在细胞因子TGF-β2联合作用下成骨分化作用更明显.

Gene X-pert MTB/RIF检测在尘肺病人中的应用

目的:探讨Gene X-pert MTB/RIF技术在尘肺病人中的应用价值。方法:对湖南省职业病防治院2020年4月1日~2022年6月30日疑似结核感染的尘肺住院患者的痰或肺泡灌洗液标本进行抗酸染色,运用Gene X-pert MTB/RIF技术检测结核分枝杆菌(Mycobacterium tuberculosis,MTB)及利福平耐药基因,使用卡方检验统计分析尘肺病人不同分期MTB阳性率的差异;利用全自动生化仪检测血清蛋白质含量,用t检验统计分析尘肺合并结核与尘肺未合并结核感染患者血清蛋白含量的差异。结果:尘肺患者中痰或肺泡灌洗液涂片抗酸染色阳性率为2.1%,Gene X-pert MTB/RIF检测MTB阳性率为5.1%,其中利福平耐药的病人占14.6%。尘肺患者不同分期三组间Gene X-pert MTB/RIF检测阳性率差异有统计学意义;尘肺合并结核感染患者白蛋白含量明显低于未合并结核感染患者,而血清总蛋白含量无明显差异。结论:Gene X-pert MTB/RIF技术可提高尘肺患者并发肺结核和利福平耐药的检出率;随着患者尘肺等级的增高,其Gene X-pert MTB /RIF 检测阳性率升高,且尘肺合并结核比未合并结核感染患者白蛋白水平降低。

Xp11.2易位/TFE3基因融合相关性肾细胞癌^(18)F-FDG PET/CT特征

目的观察Xp11.2易位/TFE3基因融合相关性肾细胞癌(Xp11.2易位肾细胞癌)PET/CT表现。方法回顾性分析6例Xp11.2易位肾细胞癌患者,观察其PET/CT表现。结果6例肿瘤最大径6.5~15.5 cm、中位最大径10.30 cm;5例呈高、低混杂密度肿块,1例呈均匀低密度;5例为囊实性、1例为实性肿块;5例^(18)F-FDG摄取增高,最大标准摄取值(SUV_(max))为2.5~6.5、中位数为6.2,1例^(18)F-FDG摄取低于相邻肾实质;5例肿瘤内或边缘可见散在点状/条状/结节状钙化灶;3例合并肾静脉/下腔静脉瘤栓,表现为静脉管腔增粗,放射性摄取增高;2例合并远处转移,分别为肺转移及肝、肺、骨多器官转移,均表现为不同程度放射性摄取增高。结论Xp11.2易位肾细胞癌PET/CT表现具有一定特征性,多呈较大软组织肿块伴囊变及钙化,^(18)F-FDG摄取多增高。

ERCC1 mRNA和X线修复交叉互补组1基因多态性联合检测在局部晚期鼻咽癌患者放化疗中的应用价值

目的 探讨核苷酸切除修复交叉互补组1(ERCC1)m RNA和X线修复交叉互补组1(XRCC1)基因多态性联合检测在局部晚期鼻咽癌患者放化疗中的应用价值。方法 选取2020年1月至2021年1月在江西省上饶市人民医院接受放化疗的41例局部晚期鼻咽癌患者,采用定量反转录聚合酶链反应检测外周血中ERCC1 mRNA的表达水平,采用限制性片段长度多态性聚合酶链反应检测XRCC1基因型(Arg194Trp、Arg280His、Arg399Gln),探讨ERCC1 mRNA和XRCC1多态性与局部晚期鼻咽癌患者放化疗效果、肿瘤复发及药物不良反应(ADR)的关系,并采用logistic回归分析局部晚期鼻咽癌患者ADR的影响因素。结果 完全缓解和部分缓解患者的ERCC1 mRNA及XRCC1多态性与疾病稳定和疾病进展患者比较差异无统计学意义(P>0.05)。肿瘤复发患者的ERCC1 mRNA及XRCC1多态性与非复发患者比较差异无统计学意义(P>0.05)。ADR患者XRCC1 Arg194Trp位点携带AG基因型、ERCC1 mRNA高表达的频率均高于非ADR患者,差异有统计学意义(P<0.05)。多因素logistic回归分析显示,XRCC1 Arg194Trp AG基因型(OR=1.876)、ERCC1mRNA高表达(OR=1.109)是局部晚期鼻咽癌患者放化疗期间发生ADR的影响因素(P<0.05)。结论 与单一检测相比,ERCC1 mRNA和XRCC1多态性联合检测预测局部晚期鼻咽癌患者放化疗期间ADR的价值更高,值得临床应用。

HBV X Gene Transfection Upregulates IL-1β and IL-6 Gene Expression and Induces Rat Glomerular Mesangial Cell Proliferation

The X gene of HBV encodes a 17-kD protein, termed HBx, which has been shown to function as a transcriptional trans-activator of a variety of viral and cellular promoter/enhancer elements. The aim of this study was to investigate the effect of HBx on gene expression of interleukin （IL）-1β and IL-6, and proliferation of rat mesangial cells in vitro. The X gene of HBV was amplified by PCR assay, and inserted into the eukaryotic expression vector pCI-neo. The structure of recombinant pCI-neo-X plasmid was proved by restrict endonuclease digestion and sequencing analysis. pCI-neo-X was transfected into cultured rat mesangial cell line in vitro via liposome. HBx expression in transfected mesangial cells was detected by Western blot. The IL-1β and IL-6 mRNA expression in those cells was assayed by semiquantitative RT-PCR. Mesangial cell proliferation was tested by MTT. The results showed that HBx was obviously expressed in cultured mesangial cell line at 36th and 48th h after transfection. The expression of IL-1β and IL-6 mRNA was simultaneously increased. The cell proliferation was also obvious at the same time. It was concluded that HBx gene transfection could induce IL-1β and IL-6 gene expression and mesangial cell proliferation. HBx may play a critical role in mesangial cell proliferation through upregulation of the IL-1β and IL-6 gene expression.

Detection of hyper-conserved regions in hepatitis B virus X gene potentially useful for gene therapy

AIM To detect hyper-conserved regions in the hepatitis B virus(HBV) X gene(HBX) 5' region that could be candidates for gene therapy.METHODS The study included 27 chronic hepatitis B treatmentnaive patients in various clinical stages(from chronic infection to cirrhosis and hepatocellular carcinoma, both HBeA g-negative and HBeA g-positive), and infected with HBV genotypes A-F and H. In a serum sample from each patient with viremia > 3.5 log IU/m L, the HBX 5' end region [nucleotide(nt) 1255-1611] was PCRamplified and submitted to next-generation sequencing(NGS). We assessed genotype variants by phylogenetic analysis, and evaluated conservation of this region by calculating the information content of each nucleotide position in a multiple alignment of all unique sequences(haplotypes) obtained by NGS. Conservation at the HBx protein amino acid(aa) level was also analyzed.RESULTS NGS yielded 1333069 sequences from the 27 samples, with a median of 4578 sequences/sample(2487-9279, IQR 2817). In 14/27 patients(51.8%), phylogenetic analysis of viral nucleotide haplotypes showed a complex mixture of genotypic variants. Analysis of the information content in the haplotype multiple alignments detected 2 hyper-conserved nucleotide regions, one in the HBX upstream non-coding region(nt 1255-1286) and the other in the 5' end coding region(nt 1519-1603). This last region coded for a conserved amino acid region(aa 63-76) that partially overlaps a Kunitz-like domain.CONCLUSION Two hyper-conserved regions detected in the HBX 5' end may be of value for targeted gene therapy, regardless of the patients' clinical stage or HBV genotype.

Possible mechanism for hepatitis B virus X gene to induce apoptosis of hepatocytes

AIM: To investigate the possible mechanism for HBV X gene to induce apoptosis of hepatocyte HL-7702 cells. METHODS: HBV X gene eukaryon expression vector pcDNA3-X was established and transfected into HL-7702 cells by Iipid-mediated transfection, including transient and stable transfection. Positive clones were screened by incubating in the selective medium with 600 μg/mL G418 and named HL-7702/HBV-encoded X protein (HBx) cells. The expressions of Fas/FasL, Bax/Bcl-2, and c-myc mRNA were measured by semi-quantitative RT-PCR in HL-7702/HBx and control group, respectively. RESULTS: RT-PCR analysis confirmed that HBV X gene was transfected into HL-7702 cells successfully. By semi-quantitative RT-PCR analysis, Bax and c-myc mRNA levels in HL-7702/HBx cells of transient transfection were significantly higher than those in control, FasL and c-myc mRNA levels in HL-7702/HBx cells of stable transfection were significantly higher than those in control, whereas the Bcl-2 mRNA levels in HL-7702/HBx cells of transient and stable transfection were significantly lower than those in control. CONCLUSION: HBV X gene may promote the apoptosis of hepatocytes by regulating the expressions of Fas/FasL, Bax/Bcl-2, and c-myc gene in a dose-dependent manner.

XRCC1 genetic polymorphism Arg399Gln and gastric cancer risk:A meta-analysis

AIM:TO evaluate the association between X-ray cross- complementing gene 1 (XRCC1) genetic polymorphism Arg399GIn and gastric cancer risk by means of meta- analysis. METHODS:We searched PubMed and NCBI up to June 1,2008.A total of 16 clinical trials and reports were identified,but only 8 trials qualified under our selection criteria.Statistical analysis was performed with the software program Review Manage,version 4.2.8. RESULTS:Of the 8 case-control studies selected for this meta-analysis,a total of 1334 gastric cancer cases and 2194 controls were included.For Arg399Gln,the Gln/Gln genotype carriers did not have a decreased cancer risk compared with those individuals with the Arg/Arg genotype (OR=0.92,95% CI,0.71-1.19; P=0.51).Similarly,no associations were found in the recessive and dominant modeling (Gln/Gln vs Arg/Gln +Arg/Arg:OR=0.96;95% CI,0.77-1.19;P=0.70 and Gln/Gln+Arg/Gln vs Arg/Arg:OR=0.90,95% CI,0.77-1.05;P=0.18). CONCLUSION:No association is found between the XRCC1 polymorphism Arg399Gln and gastric cancer risk.