多重耐药维氏气单胞菌porin基因敲除的构建及其耐药特性研究

目的研究微孔蛋白基因porin对维氏气单胞菌(Aeromonas veronii,A.veronii)耐药性的影响以解析A.veronii的耐药机制。方法以多重耐药的A.veronii WL-3为研究对象,采用同源重组双交换的方法构建Δporin敲除株,利用比浊法测定其生长曲线,通过药敏纸片法分析其耐药性。结果以A.veronii WL-3基因组DNA为模板,利用overlap聚合酶链式反应技术扩增获得上下同源臂融合片段,并连接至自杀质粒pDM4中,重组成敲除质粒pDM4-Δporin。将pDM4-Δporin转化至感受态大肠杆菌SM10中,通过接合转移转入A.veronii WL-3中。通过同源重组双交换构建A.veronii WL-3Δporin敲除株。生长曲线显示与野生株相比,Δporin菌株的生长速度并无明显变化;抗生素耐药特征分析显示敲除porin基因会降低A.veronii对头孢氨苄、新霉素、四环素、环丙沙星等10种抗生素的敏感性,提高对多粘菌素B的敏感性。结论基因porin不是A.veronii生长所必需的,但会影响A.veronii对部分抗生素的敏感度。本研究所构建的敲除株可为深入研究porin在A.veronii的耐药机制提供必要材料。

子宫肌瘤细胞中孕激素受体M、A/B及porin蛋白表达观察

目的观察子宫肌瘤细胞中孕激素受体M(PR-M)、孕激素受体A/B(PR-A/B)及porin蛋白的表达变化,并探讨其意义。方法子宫肌瘤切除术中切取子宫肌瘤组织及瘤旁正常子宫平滑肌组织后冰上尽快送实验室,原代培养子宫肌瘤细胞和正常子宫平滑肌细胞并鉴定。取第3代子宫肌瘤细胞(实验组)和正常平滑肌细胞(对照组),采用Western blotting法检测细胞中的PR-M、PR-A、PR-B、porin蛋白,分析PR-M、PR-A、PR-B蛋白与porin蛋白表达的相关性。结果实验组细胞中PR-M、PR-A、PR-B、porin蛋白相对表达量分别为0.130±0.012、0.432±0.052、0.456±0.045、0.525±0.082,对照组分别为0.086±0.015、0.223±0.036、0.269±0.026、0.202±0.034,实验组细胞中PR-M、PR-A、PR-B蛋白和porin蛋白相对表达量均高于对照组(P均<0.01)。实验组中PRM蛋白与porin蛋白相对表达量呈正相关关系(r=0.464,P<0.05)。结论子宫肌瘤细胞中PR-M、PR-A、PR-B、porin蛋白表达升高,PR-M、PR-A、PR-B、porin蛋白表达异常可能与子宫肌瘤的发病有关,且PR-M蛋白与porin蛋白可能在子宫肌瘤发病中起协同作用。

子宫平滑肌瘤组织中孕激素受体和porin mRNA的表达

目的:探讨孕激素促进子宫平滑肌瘤形成的机制。方法:采用RT-PCR方法检测28例子宫平滑肌瘤组织(研究组)和瘤旁正常子宫平滑肌组织(对照组)中新型孕激素受体(PR)-M、PR-A、PR-B和线粒体porin mRNA的表达。结果:研究组PR-M、porin、PR-A和PR-B mRNA的表达均高于对照组(t=23.935、12.881、10.059和9.332,P<0.001);研究组中PR-M和porin mRNA的表达呈正相关(r=0.431,P=0.022)。结论:PR-M可能通过非基因组途径参与子宫平滑肌瘤的形成。

鼠伤寒沙门氏菌porin蛋白免疫原性的研究

用从鼠伤寒沙门氏菌（STM）中提取的微孔蛋白porin免疫BALB／c小鼠，不仅能产生高效价的抗体，还能出现典型的迟发型变态反应（DTH）和白细胞介素－2（IL－2）。以500LD50鼠伤寒沙门氏菌攻击，其保护率为70％，提示STM－porin具有较强的免疫原性。

鼠伤寒沙门氏菌外膜蛋白(porin)的提纯及鉴定

采用超声破碎、TritonX－100溶解、Sephacryl超细S－300和SephadexG－150凝胶过滤提纯了鼠伤寒杆菌的外膜蛋白porin。经检测其中LPS的含量约为0．06％。经SDS—PAGE图谱分析，porin在36KDa位置处显示一条蛋白带；用免疫印迹将OMPs兔抗血清与porin结合，仅在36KDa位置显示一明显的印迹带。

鼠伤寒沙门氏菌porin诱导BALB/c小鼠细胞免疫的研究

目的 探讨鼠伤寒沙门氏菌 porin(STM- porin)诱导 BAL B/ c小鼠细胞免疫的能力。方法 迟发型变态反应(DTH)、IL - 2分别采用足垫肿胀、MTT法 ;利用尼龙毛柱纯化免疫的 BAL B/ c小鼠的 T淋巴细胞通过尾静脉转移到非免疫小鼠 ,再用 5 0 0 L D5 0 的 STM攻击。结果 用 STM- porin免疫的 BAL B/ c小鼠可以产生较高水平的 DTH (3.6± 0 .2 ,P<0 .0 1)和IL - 2 (2 6 .2± 4.9,P<0 .0 1) ;同时 T淋巴细胞被动免疫保护 (42 .9% )也明显高于 L PS组 (0 % ) ,P<0 .0 1。结论 这些结果说明 STM- porin可能诱导 BAL B/

淋球菌外膜蛋白Porin I多抗的黏附抑制作用研究

目的:研究兔抗淋球菌外膜蛋白Porin I(P I)的多克隆抗体阻断淋病奈瑟菌对泌尿生殖道上皮的黏附作用。方法:将自行构建表达的淋球菌GST-P I融合蛋白作为抗原免疫新西兰兔,获得兔抗P I蛋白的多抗血清,纯化后得到P I-IgG抗体。建立淋球菌感染BALB/c小鼠模型,并通过观察阴道黏膜改变、分泌物涂片、冲洗液培养及阴道组织病理变化评价兔抗P I-IgG抗体对淋球菌黏附的影响。结果:经1 m g/m l兔抗P I-IgG处理后3 h再接种淋球菌的BALB/c小鼠生殖道黏膜未见红肿及脓液,分泌物涂片及阴道冲洗液未检及淋球菌,阴道组织病理检查也未见炎症细胞浸润。而低于浓度1 m g/m l及长于3 h兔抗P I-IgG处理的小鼠阴道组织病理可检及炎症细胞,但其它检查结果阴性。结论:纯化的抗淋球菌GST-P I融合蛋白的多克隆抗体,能有效抑制淋病奈瑟菌对小鼠泌尿生殖道上皮的黏附与感染,阻断作用及持续时间与抗体浓度有关。

鼠伤寒沙门氏菌porin诱导BALB/C小鼠迟发性变态反应和T淋巴细胞转移保护的研究

[目的 ] 探讨鼠伤寒沙门氏菌porin(STM -porin)诱导BALB/C小鼠迟发性变态反应和T淋巴细胞转移保护的能力。 [方法 ] 迟发型变态反应 (DTH) ,采用足垫肿胀法 ;利用尼龙毛柱纯化免疫BALB/C小鼠的T淋巴细胞通过尾静脉转移到非免疫小鼠 ,再用 5 0 0LD50 的STM攻击。 [结果 ] 用STM -porin免疫的BABL/C小鼠可以产生明显的DTH ;同时T淋巴细胞被动免疫保护也明显高于LPS组 (P <0 0 1)。 [结论 ] 结果说明STM -porin可能诱导BALB/C小鼠产生较强的DTH和T淋巴细胞免疫保护。

Helicobacter pylori HopE and HopV porins present scarce expression among clinical isolates

AIM:To evaluate how widely Helicobacter pylori (H. pylori ) HopE and HopV porins are expressed among Chilean isolates and how seroprevalent they are among infected patients in Chile.METHODS: H. pylori hopE and hopV genes derived from strain CHCTX-1 were cloned by polymerase chain reaction (PCR), sequenced and expressed in Escherichia coli AD494 (DE3). Gel-purified porins were used to prepare polyclonal antibodies. The presence of both genes was tested by PCR in a collection of H. pylori clinical isolates and their expression was detected in lysates by immunoblotting. Immune responses against HopE, HopV and other H. pylori antigens in sera from infected and non-infected patients were tested by Western blotting using these sera as f irst antibody on recombinant H. pylori antigens.RESULTS: PCR and Western blotting assays revealed that 60 and 82 out of 130 Chilean isolates carried hopE and hopV genes, respectively, but only 16 and 9, respectively, expressed these porins. IgG serum immunoreactivity evaluation of 69 H. pylori-infected patients revealed that HopE and HopV were infrequently recognized (8.7% and 10.1% respectively) compared to H. pylori VacA (68.1%) and CagA (59.5%) antigens. Similar values were detected for IgA serum immunoreactivity against HopE (11.6%) and HopV (10.5%) although lower values for VacA (42%) and CagA (17.4%) were obtained when compared to the IgG response.CONCLUSION: A scarce expression of HopE and HopV among Chilean isolates was found, in agreement with the infrequent seroconversion against these antigens when tested in infected Chilean patients.

淋病奈瑟球菌表面Porin B蛋白特异性及免疫保护性临床应用价值分析

目的研究淋病奈瑟球菌(NG)表面Porin B(Por B)蛋白特异性及免疫保护性在临床中的应用价值。方法登录Gen Bank获取NG世界卫生组织(WHO)标准株E株Por B-PIA基因,设计引物与合成,培养WHO标准株E株,通过聚合酶链反应(PCR)扩增出Por B-PIA DNA片段,采用GST·Bind^(TM)树脂纯化Por B蛋白,对噬菌体随机12肽库进行筛选并对阳性克隆进行提取,应用DNA测序及MIXOX软件分析;将培养后的人尿道上皮细胞分别与Por B蛋白特异性结合的多肽、NG活菌进行培养,并将未加入抗体作为对照组。观察Por B蛋白的纯化表达,Western blot检测Por B蛋白与NG特异性关系,间接酶联免疫吸附试验(ELISA)检测筛选后蛋白的特异性抗体水平,比较Por B蛋白特异性结合多肽对细胞内形成微菌落的差异。结果Ecoli-BL21中克隆表达的诱导产物经Ni+-NTA Purification System纯化后,获得纯度较高的Por B蛋白;制备出Por B蛋白相应的特异性结合多肽,蛋白出现特异性条带;间接ELISA检测筛选后蛋白的特异性抗体水平,筛选后蛋白的抗体水平在1∶200;加入Por B蛋白特异性结合多肽的组形成的微菌落显著少于对照组(P<0.05)。结论NG表面Por B蛋白发挥显著特异性和免疫保护性,但还需大量研究及临床试验来证明其临床效果并进一步分析Por B蛋白的相关机制和作用,为临床NG疫苗的研究提供依据。

Stable Surface Expression of a Gene for Helicobacter pylori Toxic Porin Protein with pBAD Expression System

Helicobacter pylori(H.pylori)infection causes peptic and duodenal diseases in humans. Among a 32-protein family of outer membrane proteins,a porin-like protein,HopE,has been a subject of note,mainly for its conservative nature among H.pylori,and for its potential as a vaccine candidate.To achieve stable surface expression of this host cell-toxic protein,hopE gene was introduced into pBAD expression system.After induction with arabinose,all 15 randomly-chosen E.coli LMG 194 colonies from 3 successive passages could express HopE protein,while only 1 from 5 E.coli colonies that contained lac operon-regulated plasmid encoding hopE gene could express HopE.Indirect immunofluorescence confirmed the expression of HopE on E.coli cell surface.

Construction of Prokaryotic Expression Plasmid of Fusion Protein Including Porin A and Porin B of Neisseria Gonorrhoeae and Its Expression in E.coli

In order to provide a rational research basis for clinical detection and genetic engineering vaccine, plasmid pET-28a (+) encoding both Porin gene PIA and PIB of Neisseria gonorrhoeae was constructed and a fusion protein in E.coli DE3 expressed. The fragments of PIA and PIB gene of Neisseria gonorrhoeae were amplified and cloned into prokaryotic expression plasmid pET-28a(+) with double restriction endonuclease cut to construct recombinant pET-PIB-PIA. The recombinant was verified with restriction endonuclease and sequenced and transformed into E.coli DE3 to express the fusion protein PIB-PIA after induced with IPTG. The results showed PIA-PIB fusion DNA fragment was proved correct through sequencing. A 67 kD (1 kD=0 992 1 ku) fusion protein had been detected by SDS-PAGE. It was concluded that the fusion protein was successively expressed.

Construtcion of Neisseria Gonorrhoeae Porin B Plasmid Recombinant and Its Expression in E.coli

A prokaryotic expression recombinant plasmid pET-PIB to express porin B （PIB） of Neisseria gonorrhoeae in E.coli DE3 was constructed in order to provide a basis of research in detection, prophylactic and therapeutic vaccine against the pathogen infection. The gene encoding PIB was amplified by PCR from Neisseria gonorrhoeae and cloned into prokaryotic expression plasmid pET-28a（+） to construct a pET-PIB recombinant, which was verified by restriction endonuclease and DNA sequencing. Protein PIB was expressed in E.coli DE3 induced with IPTG. The antigenicity of the expressed protein was evaluated by indirect ELISA. Rabbits were immunized with the protein and serum was collected after immunization. To assess the immunogenicity of the protein, the titer of serum to protein PIB was determined by ELISA. DNA sequence analysis showed that the nucleic acid sequence of PIB gene was 99.28 % of homology compared with that （NGPIB18） published in GenBank. A 41 kD fused protein was detected by SDS-PAGE and was proven to have reactivity with anti-PIB polyclonal antibody from mouse. A polyclonal antibody to PIB of 1:4000 titer determined by indirect ELISA was obtained from rabbit immunized with the purified product. Recombinant plasmid encoding PIB of Neisseria gonorrhoeae was constructed. Protein PIB with antigenicity and immunogenicity was successfully expressed.

鸭疫里默氏杆菌Porin蛋白的原核表达及其间接ELISA检测方法的建立与应用

旨在建立一种新型可适用于鸭疫里默氏杆菌(RA)病抗体检测的间接ELISA方法。以血清2型RA贵州分离株为研究对象,将其微孔蛋白Proin编码的基因克隆至pET-32a载体,构建重组表达质粒pET-32a-porin,在E.coli BL21(DE3)中使用IPTG诱导后表达。以纯化后的Porin蛋白作为包被抗原,通过一系列条件的优化建立一种检测RA抗体的间接ELISA方法,对其性能进行综合评价。结果显示,该方法具有较好的敏感性、重复性及特异性,阳性血清经1∶6 400稀释后检测结果仍为阳性,批内变异系数(CV)在1.27%~4.90%之间,批间CV在2.59%~5.43%之间,该方法可特异性地检测出抗RA抗体,与禽流感病毒(AIV)H5亚型、AIV H7亚型、新城疫病毒(NDV)、鸭圆环病毒(DuCV)、鸭坦布苏病毒(DTMUV)及E.coli阳性血清均无交叉反应,与商品化ELISA抗体试剂盒检测相比,两者符合率为97.26%。使用建立的ELISA方法对临床采集的801份样品血清开展抗体检测分析(626份为已免疫鸭传染性浆膜炎二价灭活疫苗“血清1型+血清2型”的样品血清,175份为未免疫任何鸭传染性浆膜炎疫苗的样品血清),有564份为免疫抗体阳性,检出阳性率为90.01%(564/626),有36份为感染抗体阳性,检出阳性率为20.99%(36/175)。结果表明,本研究建立了一种新型可用于RA抗体检测的间接ELISA方法,为RA的血清学流行病学调查提供了新的检测方法。

浙江地区奈瑟淋球菌临床菌株porinⅠ基因优势型及原核表达系统的构建

目的分析浙江地区奈瑟淋球菌临床菌株porinⅠ基因优势型分布情况,构建porinⅠA与porinⅠB基因的原核表达系统。方法在先前研究的基础上,对确定的porinⅠA和porinⅠB基因进行T-A克隆后测定核苷酸顺序,分析porinⅠA和porinⅠB的地区优势基因型。再构建porinⅠA和porinⅠB基因优势基因型的原核表达系统,0.5 mmo L/L IPTG诱导后,10%SDS-PAGE检测蛋白表达情况。结果测序的5株porinⅠA全为血清型ⅠA-6;测序的11株porinⅠB中,血清型ⅠB-3有5株,血清型ⅠB-3/6有3株,血清型ⅠB-6有1株,其余2株为变异株。构建的原核表达系统PET-42-PⅠA的PⅠA表达量占细菌总蛋白量的30%;PET-42-PⅠB的PⅠB表达量占细菌总蛋白量的20%。结论浙江地区奈瑟淋球菌临床菌株porinⅠA以血清型ⅠA-6为优势基因型,porinⅠB以血清型ⅠB-3为优势基因型,porinⅠA相对于porinⅠB而言更加保守。所构建的原核表达系统能高效表达PⅠA与PⅠB重组蛋白。

Deletion of Mitochondrial Porin Alleviates Stress Sensitivity in the Yeast Model of Shwachman-Diamond Syndrome

Shwachman-Diamond syndrome(SDS) is a multi-system disorder characterized by bone marrow failure, pancreatic insufficiency,skeletal abnormalities, and increased risk of leukemic transformation. Most patients with SDS contain mutations in the ShwachmanBodian-Diamond syndrome gene(SBDS), encoding a highly conserved protein that has been implicated in ribosome biogenesis.Emerging evidence also suggests a distinct role of SBDS beyond protein translation. Using the yeast model of SDS, we examined the underlying mechanisms that cause cells lacking Sdo1 p, the yeast SBDS ortholog, to exhibit reduced tolerance to various stress conditions.Our analysis indicates that the environmental stress response(ESR), heat shock response(HSR), and endoplasmic reticulum unfolded protein response(UPR) of sdo1 D cells are functional and that defects in these pathways do not produce the phenotypes observed in sdo1 D yeast. Depletion of mitochondrial DNA(mt DNA) was observed in sdo1 D cells, and this is a probable cause of the mitochondrial insufficiency in SDS. Prior disruption of POR1, encoding the mitochondrial voltage dependent anion channel(VDAC), abrogated the effects of SDO1 deletion and substantially restored resistance to environmental stressors and protected against damage to mt DNA.Conversely, wild-type cells over-expressing POR1 exhibited growth impairment and increased stress sensitivity similar to that seen in sdo1 D cells. Overall, our results suggest that specific VDAC inhibitors may have therapeutic benefits for SDS patients.

2016-2018年东莞地区耐碳青霉烯类肠杆菌目细菌的耐药表型、耐药机制和分子流行病学分析

目的通过研究东莞地区的耐碳青霉烯类肠杆菌目细菌(carbapenem-resistant Enterobacteriaceae,CRE)的耐药情况和基因分型,研究耐碳青霉烯类肺炎克雷伯菌(carbapenem-resistant Klebsiella pneumoniae,CRKP)的亲缘性、耐药机制和bla_(KPC-2)基因环境,为临床寻找控制和治疗该致病菌的更优方案提供参考。方法回顾性收集2016年1月—2018年12月东莞市人民医院、东莞东华医院、康华医院、东莞市中医院和东莞市妇幼保健院等十三所医院的住院患者的CRE菌株进行常规微生物培养、鉴定和药敏试验。以美罗培南或亚胺培南纸片法(K-B法)或最小抑菌浓度(MIC)测定法对肠杆菌目细菌进行初筛;采用改良Hodge试验、亚胺培南-EDTA双纸片协同试验和CIM试验检测CRE产酶情况;聚合酶链式反应(polymerase chain reaction,PCR)检测并鉴定CRE的碳青霉烯类耐药基因(bla_(KPC)、bla_(NDM)、bla_(IMP)、bla_(DHA)、bla_(CTX-M)和bla_(CMY)),以及CRKP的多位点序列分型(multilocus sequence typing,MLST)和孔蛋白(OmpK35、OmpK36和OmpK37);通过Junction PCR、Mapping PCR和Crossing PCR检测bla_(KPC-2)基因环境;使用WHONET 5.6软件统计分析CRE临床分离株在标本和科室中的分布与耐药情况,以及碳青霉烯酶基因在科室中的分布情况。结果从37217株肠杆菌目细菌中共检出131株CRE(占0.35%),其中肺炎克雷伯菌79株(占60.31%)、大肠埃希菌21株(占16.03%)和阴沟肠杆菌12株(占9.16%);检出CRE的临床科室主要为ICU(66株,占50.38%);在检出CRE的标本中,位于前3位分别是痰液标本(56株,占42.75%)、尿液标本(21株,占16.03%)、伤口分泌物标本(12株,占9.16%);CRE对目前临床中常使用的抗菌药物表现出高耐药性,仅对阿米卡星耐药率较低,为21.38%。检测104株CRE(包括肺炎克雷伯菌、大肠埃希菌和阴沟肠杆菌)发现的碳青霉烯酶有KPC-2型(57,54.81%)、NDM-1型(7株,6.73%)和NDM-5型(2株,1.92%);其中,CRKP主要为ST11型(49株,占62.03%),其次为ST1型(25株,占31.65%);ompK35(75株,占94.94%)、ompK36(77株,占97.47%)和ompK37(79株,占100%)发生突变的占比高;bla_(KPC-2)的基因环境主要为B1型突变型(38株,占48.10%),其次为A型突变型(14株,占17.72%)。结论2016—2018年东莞地区临床CRE检出率为0.35%,耐药性强,其中,CRKP主要为ST11型,主要流行的是KPC-2型,其基因环境为B1型突变型,而且孔蛋白突变占比极高,这提示东莞地区bla_(KPC-2)基因主要通过质粒进行传播,并且孔蛋白突变在CRE中发挥重要作用,院内感染医务工作者应根据该菌科室分布、耐药情况和耐药机制等特点,采取合理有效的预防和治疗方法。

肺炎克雷伯菌产KPC酶合并膜孔蛋白OmpK36缺失对头孢他啶/阿维巴坦耐药的分子机制研究

目的研究产KPC酶肺炎克雷伯菌(Klebsiella pneumoniae,Kp)对头孢他啶/阿维巴坦耐药的分子机制。方法临床分离2株对头孢他啶/阿维巴坦耐药的产KPC酶Kp C9和C14,利用胶体金法进行碳青霉烯酶型检测,基质辅助激光解吸飞行时间质谱(MALDI-TOF MS)进行同源性分析,MIC法进行药物最低抑菌浓度检测,聚丙烯酰胺凝胶电泳(SDS-PAGE)及基因测序检测外膜蛋白表达及基因突变,羰基氰化物间氯苯腙(CCCP)抑制试验检测主动外排机制。结果产KPC酶Kp C9和C14同其他产KPC酶Kp同源性较低,对头孢他啶/阿维巴坦的MIC分别为16和32μg/mL,外膜蛋白SDS-PAGE显示Kp C9和C14均有OmpK36的缺失,外膜蛋白基因序列分析显示Kp C9和C14的OmpK36基因序列均存在个别位点的突变、缺失,CCCP抑制试验显示CCCP不能提高Kp C9和C14对头孢他啶/阿维巴坦的敏感性。结论KPC酶合并膜孔蛋白OmpK36缺失可引起Kp对头孢他啶/阿维巴坦耐药。

结肠癌患者组织中NCAPD2、Lnc RNA NR2F1-AS1、Nup107表达及其与预后的关系

目的探究结肠癌患者组织中染色体凝缩蛋白复合物I的亚基D2(NCAPD2)、Lnc RNA核受体亚家族2F组成员1-反义RNA1(Lnc RNA NR2F1-AS1)、核孔蛋白107(Nup107)的表达及其与患者预后的关系。方法选择2017年6月至2019年6月在广州中医药大学第一附属医院及暨南大学附属广州市红十字会医院进行根治性切除术的60例结肠癌患者作为研究对象,术中采集患者的结肠癌组织标本和距离结肠癌组织>2 cm的癌旁正常组织标本。采用实时荧光定量PCR(RT-PCR)法测定结肠癌组织和癌旁组织的Lnc RNA NR2F1-AS1表达水平,采用免疫组化SP法测定结肠癌组织和癌旁组织的NCAPD2和Nup107表达情况。比较结肠癌组织和癌旁组织的Lnc RNA NR2F1-AS1、NCAPD2、Nup107表达情况,同时比较Lnc RNA NR2F1-AS1、NCAPD2、Nup107不同表达患者的临床资料。采用COX回归模型分析Lnc RNA NR2F1-AS1、NCAPD2、Nup107表达对结肠癌患者预后的影响,采用Kaplan-Meier法绘制结肠癌患者的生存曲线,分析Lnc RNA NR2F1-AS1、NCAPD2、Nup107表达情况与结肠癌患者预后的相关性。结果结肠癌组织的Lnc RNA NR2F1-AS1相对表达量为1.09±0.28,明显低于癌旁组织的0.69±0.09,结肠癌组织的Lnc RNA NR2F1-AS1高表达率、NCAPD2阳性率和Nup107高表达率分别为55.00%、61.67%和70.00%,明显高于癌旁组织的26.67%、30.00%和31.67%,差异均有统计学意义(P<0.05);Lnc RNA NR2F1-AS1高表达和低表达患者、NCAPD2阳性患者和阴性患者、Nup107高表达患者和低表达患者在肿瘤分化程度、浸润程度、淋巴结转移和远端转移方面比较,差异均有统计学意义(P<0.05);COX回归分析结果显示,Lnc RNA NR2F1-AS1、NCAPD2和Nup107表达均是结肠癌患者预后的影响因素(P<0.05);Kaplan-Meier生存曲线分析结果显示,Lnc RNA NR2F1-AS1高表达、NCAPD2阳性和Nup107高表达患者的中位生存期分别低于Lnc RNA NR2F1-AS1低表达、NCAPD2阴性和Nup107低表达患者,差异均有统计学意义(P<0.05)。结论Lnc RNA NR2F1-AS1、NCAPD2、Nup107的表达与结肠癌患者的肿瘤分化程度、浸润程度、淋巴结转移和远端转移等临床病理特征有关,三者可能共同参与了结肠癌的发生、发展,对患者的预后造成一定影响。