Fusion protein of single-chain variable domain fragments for treatment of myasthenia gravis

Single-chain variable domain fragment （scFv） 637 is an antigen-specific scFv of myasthenia gravis. In this study, scFv and human serum albumin genes were conjugated and the fusion pro-tein was expressed in Pichia pastoris. The afifnity of scFv-human serum albumin fusion protein to bind to acetylcholine receptor at the neuromuscular junction of human intercostal muscles was detected by immunolfuorescence staining. The ability of the fusion protein to block myas-thenia gravis patient sera binding to acetylcholine receptors and its stability in healthy serum were measured by competitive ELISA. The results showed that the inhibition rate was 2.0-77.4%, and the stability of fusion protein in static healthy sera was about 3 days. This approach suggests the scFv-human serum albumin is a potential candidate for speciifc immunosuppressive therapy of myasthenia gravis.

Inhibitory effect of endostatin expressed by human liver carcinoma SMMC7721 on endothelial cell proliferation in vitro

AIM: To construct a stable transfectant of human liver carcinoma cell line SMMC7721 that could secret human endostatin and to explore the effect of human endostatin expressed by the transfectant on endothelial cell proliferation. METHODS: Recombinant retroviral plasmid pLncx-Endo containing the cDNA for human endostatin gene together with rat albumin signal peptide was engineered and transferred into SMMC7721 cell by lipofectamine. After selection with G418, endostatin-transfected SMMC7721 cells were chosen and expanded. Immunohistochemical staining and Western blot were used to detect the expression of human endostatin in transfected SMMC7721 cells and its medium. The conditioned medium of endostatin-transfected and control SMMC7721 cells were collected to cultivate with human umbilical vein endothelial cells for 72 hours. The inhibitory effect of endostatin, expressed by transfected SMMC7721 cells, on endothelial proliferation in vitro was observed by using MTT assay. RESULTS: A 550 bp specific fragment of endostatin gene was detected from the PCR product of endostatin-transfected SMMC7721 cells. Immunohistochemistry and Western blot analysis confirmed the expression and secretion of foreign human endostatin protein by endostatin-transfected SMMC7721 cells. In vitro endothelial proliferation assay showed that 72 hours after cultivation with human umbilical vein endothelial cells, the optical density (OD) in group using the medium from endostatin-transfected SMMC7721 cells was 0.51 +/- 0.06, lower than that from RPMI 1640 group (0.98 +/- 0.09) or that from control plasmid pLncx-transfected SMMC7721 cells (0.88 +/- 0.11). The inhibitory rate for medium from endostatin-transfected SMMC7721 cells was 48%, significantly higher than that from empty plasmid pLncx-transfected SMMC7721 cells (10.2%, P【0.01). CONCLUSION: Human endostatin can be stably expressed by SMMC7721 cell transferred with human endostatin gene and its product can significantly inhibit the proliferation of human umbilical vein endothelial cell in vitro.

Expression and identification of recombinant soluble single-chain variable fragment of monoclonal antibody MC3

AIM: To generate soluble single chain variable fragments (ScFv) of monoclonal antibody MC3 recognizing colorectal and gastric carcinomas. METHODS: mRNA was isolated from the hybridoma cell line producing MC3 and the DNAs encoding variable domains of heavy and light chains (VH and VL) of the antibody were amplified separately by RT-PCR and assembled into ScFv DNA with a linker DNA. The ScFv DNA was ligated into the phagemid vector pCANTAB5E and the ligated sample was transformed into E.coli TG1.The transformed cells were infected with M13KO7 helper phage to yield recombinant phages. After two rounds of panning with gastric carcinoma cell line AGS highly expressing MC3-binding antigen, the phage clones displaying ScFv fragments of the antibody were selected by ELISA. 4 phage clones showing strong signal in ELISA were used to infect E.coli HB2151 to express soluble ScFvs. The soluble ScFvs were identified by Dot blot and Western blot, and their antigen-binding activity was assayed by ELISA. The VH and VL DNAs of the ScFv DNA derived from phage clone 19 were sequenced. RESULTS: The VH,VL and ScFv DNAs were about 340 bp, 320 bp and 750 bp respectively. After two rounds of panning to the recombinant phages, 18 antigen-positive phage clones were selected from 30 preselected phage clones by ELISA. All the soluble ScFvs derived from the 4 out of the 18 antigen-positive phage clones were about M(r)32000 and concentrated in periplasmatic space under the given culture condition. The soluble ScFvs could bind the antigen, and they shared the same binding site with MC3. The sequences of the VH and VL DNAs of the MC3 ScFv showed that the variable antibody genes belonged to the IgG1 subgroup,kappa-type. CONCLUSION: The soluble ScFv of MC3 is successfully produced, which not only provides a possible novel targeting vehicle for in vivo and in vitro study on associated cancers, but also offers the antibody a stable genetic source.

Identification of the epitopes on HCV core protein recognized by HLA-A2 restricted cytotoxic T lymphocytes

AIM: To identify hepatitis C virus(HCV) core protein epitopes recognized by HLA-A2 restricted cytotoxic T lymphocyte (CTL). METHODS: Utilizing the method of computer prediction followed by a 4h(51)Cr release assay confirmation. RESULTS: The results showed that peripheral blood mononuclear cells (PBMC) obtained from two HLA-A2 positive donors who were infected with HCV could lyse autologous target cells labeled with peptide "ALAHGVRAL (core 150-158)". The rates of specific lysis of the cells from the two donors were 37.5% and 15.8%, respectively. Blocking of the CTL response with anti-CD4 mAb caused no significant decrease of the specific lysis. But blocking of CTL response with anti-CD8 mAb could abolish the lysis. CONCLUSION: The peptide (core 150-158) is the candidate epitope recognized by HLAA2 restricted CTL.

Altered expression of nuclear matrix proteins in etoposide induced apoptosis in HL-60 cells

The events of cell death and the expression of nuclear matrix protein (NMP) have been investigated in a promyelocytic leukemic cell line HL-60 induced with etoposide. By means of TUNEL assay, the nuclei displayed a characteristic morphology change, and the amount of apoptotic cells increased early and reached maximun about 39% after treatment with etoposide for 2 h. Nucleosomal DNA fragmentation was observed after treatment for 4 h. The morphological change of HL-60 cells, thus, occurred earlier than the appearance of DNA ladder. Total nuclear matrix proteins were analyzed by 2-dimensional gel electrophoresis. Differential expression of 59 nuclear matrix proteins was found in 4 h etoposide treated cells. Western blotting was then performed on three nuclear matrix acssociated proteins, PML, HSC70 and NuMA. The expression of the suppressor PML protein and heat shock protein HSC70 were significantly upregulated after etoposide treatment, while NuMA, a nuclear mitotic apparatus protein, was down regulated. These results demonstrate that significant biochemical alterations in nuclear matrix proteins take place during the apoptotic process.

血清CYFRA21-1、CEA、SCC、HE4、ProGRP对肺癌早期诊断及病理类型鉴别的临床价值

目的探究肿瘤标志物血清细胞角蛋白19片段(CYFRA21-1)、癌胚抗原(CEA)、鳞状细胞癌抗原(SCC)、人附睾蛋白4(HE4)、胃泌素释放肽前体(ProGRP)对肺癌早期诊断及病理类型鉴别的临床价值。方法选取2021年2月至2022年2月安康市中心医院收治的280例肺癌早期患者作为肺癌组,同期收治的100例肺部良性疾病患者作为良性对照组,比较两组患者的血清CYFRA21-1、CEA、SCC、HE4及ProGRP水平,采用受试者工作特征曲线(ROC)分析血清CYFRA21-1、CEA、SCC、HE4、Pro GRP以及联合检测对肺癌早期诊断的临床价值,并根据肺癌组患者的病理分型结果比较非小细胞肺癌(NSCLC)与小细胞肺癌(SCLC)患者的血清CYFRA21-1、CEA、SCC、HE4及ProGRP水平。结果肺癌组患者的血清CYFRA21-1、CEA、SCC、HE4及ProGRP水平分别为(2.04±1.87)ng/mL、(3.08±0.82)ng/mL、(4.51±1.54)ng/mL、(60.14±15.88)pmol/L、(61.27±19.34)μg/L,明显高于良性对照组的(1.15±0.43)ng/mL、(2.54±0.71)ng/mL、(3.09±1.68)ng/mL、(45.14±17.56)pmol/L、(50.14±18.73)μg/L,差异均有统计学意义(P<0.05);经ROC分析结果显示,血清CYFRA21-1诊断肺癌早期的最佳截断值为1.830 ng/m L,CEA为2.856 ng/mL,SCC为3.140 ng/mL,HE4为50.340 pmol/L,ProGRP为57.605μg/L,5项指标联合诊断肺癌早期的AUC及敏感度达到0.901、89.30%,均高于单一指标诊断,差异有统计学意义(P<0.05);SCLC组患者的ProGRP水平明显高于NSCLC组,差异有统计学意义(P<0.05),而两组患者的CYFRA21-1、CEA、SCC及HE4水平比较差异均无统计学意义(P>0.05);腺癌组患者的SCC为(5.50±2.73)ng/mL,明显高于鳞癌组的(1.42±0.05)ng/mL,差异有统计学意义(P<0.05),而两组患者的CYFRA21-1、CEA、HE4及ProGRP水平比较差异均无统计学意义(P>0.05)。结论与肺部良性疾病患者比较,肺癌早期患者血清CYFRA21-1、CEA、SCC、HE4及ProGRP水平更高,且其联合检测诊断早期肺癌的临床价值高,血清ProGRP鉴别NSCLC与SCLC,血清SCC鉴别腺癌与鳞癌均有一定价值,建议临床密切监测。

中性粒细胞与淋巴细胞比值、细胞角蛋白19片段及人附睾蛋白4检测在子宫内膜癌诊断中的应用

目的探讨中性粒细胞与淋巴细胞比值(NLR)、细胞角蛋白19片段(CYFRA21-1)及人附睾蛋白4(HE4)检测在子宫内膜癌诊断中的应用。方法选取52例子宫内膜癌患者作为子宫内膜癌组,同期收治的50例子宫良性病变患者作为子宫良性病变组。检测两组患者NLR、CYFRA21-1及HE4水平,采用受试者工作特征曲线(ROC)分析上述指标对子宫内膜癌的诊断效能。结果子宫内膜癌组患者的血清NLR、CYFRA21-1及HE4水平均高于子宫良性病变组(P<0.01);ROC曲线分析显示,血清NLR、CYFRA21-1及HE4联合检测子宫内膜癌的诊断效能最高(AUC为0.935),其次为NLR(AUC为0.703)。结论血清NLR、CYFRA21-1及HE4在子宫内膜癌中表达水平较高,三者联合检测时诊断效能最高。

人源噬菌体抗体库的构建及抗人NH-LBP抗体的筛选与鉴定

目的: 构建人源噬菌体抗体库并制备抗人脂多糖结合蛋白氨基端片段 (NH- LBP)的单克隆抗体 (mAb)。方法:以噬菌体展示系统(pComb3H/VCSM13)建立人源噬菌体抗体库(Fab), 并以昆虫细胞sf21在无血清培养基 (SF 900Ⅱ )中,通过BAC- TO- BAC杆状病毒表达系统来表达NH -LBP。再以NH -LBP为抗原, 从人源噬菌体抗体库中筛选可产生抗NH- LBPmAb的菌株并进行鉴定。结果: 昆虫细胞sf21可表达人源NH- LBP, 经亲和纯化柱芯 (TALON)有效纯化后, 获得约8mg的NH- LBP。成功地建立人源噬菌体抗体库, 库容达5. 0×108 CFU。经 8轮筛选后, 抗体库被富集 1. 85×104 倍。经ELISA法鉴定, 获得 3株可产生抗NH -LBPmAb的菌株(核酸序列及氨基酸序列见GenBank中的: AY337713,AY337714 )。结论: 以昆虫细胞sf21表达NH LBP及以其为抗原制备噬菌体mAb是可行的。本研究为进一步建立抗NH- LBP的二硫键稳定的Fv抗体 ( disulfidestabilizedFvfrag ments, dsFv), 研究人体内LBP的变化规律和过度炎症反应的防治奠定了基础。

HE4、CYFRA21-1和TPS联合检测对非小细胞肺癌的早期诊断价值

目的：探讨血清肿瘤标志物人附睾蛋白4（HE4）、细胞角蛋白19片段（CYFRA21-1）和组织多肽特异性抗原（TPS）联合检测在非小细胞肺癌（NSCLC）早期诊断中的应用价值。方法：应用电化学发光法和ELISA分别测定NSCLC患者、肺部良性病变患者及健康对照组人员血清中HE4、CYFRA21-1和TPS水平．比较3组间HE4、CYFRA21—1和TPS水平与阳性率的差异．以及联合检测诊断NSCLC的敏感性及特异性。结果：（1）肺癌患者整体TPS、CYFRA21-1和HE4水平及I～Ⅱ期NSCLC患者HE4水平显著高于肺部良性病变患者及健康体检者（P〈0．05）；Ⅲ～Ⅳ期NSCLC患者TPS、CYFRA21-1和HE4水平高于I-ⅡNSCLC患者（P〈0．05）。（2）HE4、CYFRA21—1和TPS联合检测诊断NSCLC的敏感性较单项检测敏感性明显增高（P〈0．05）。结论：血清HE4检测比CYFRA21．1和TPS对于NSCLC有更高的早期诊断价值。血清HE4、CYFRA2I-1和TPS联合检测对于NSCLC的诊断较单一指标具有更高的诊断价值。

血清肿瘤标志物HE4对肺癌的诊断价值

目的探讨血清肿瘤标志物人附睾蛋白4(human epididymis,HE4)对肺癌的诊断价值。方法以80例肺癌患者为病例组,30例肺部良性疾病患者为良性对照组,30例健康人为健康对照组,检测所有研究对象的血清癌胚抗原(CEA),细胞角蛋白片段21-1(CYFRA21 1),神经元特异性烯醇化酶(NSE)和HE4水平。结果病例组血清CEA,NSE,CYFRA21-1和HE4水平均高于良性对照组或健康对照组(P<0.05)。四种标志物诊断肺癌患者的受试者工作特征曲线(ROC曲线)下面积(AUC)分别为0.870,0.818,0.746和0.897。腺癌患者血清CEA和HE4,鳞癌患者血清CYFRA21-1,小细胞肺癌(SCLC)患者血清NSE水平较高(P<0.05)。血清CYFRA21-1(AUC=1.000),CEA(AUC=0.727)和HE4(AUC=0.622)水平检测对鳞癌诊断有价值(P<0.05),血清CEA(AUC=0.954)和HE4(AUC=0.944)水平检测对腺癌诊断有价值(P<0.05),检测血清NSE(AUC=0.876)水平对SCLC诊断有价值(P<0.05)。结论肺癌患者血清HE4,CEA,NSE和CYFRA21-1等肿瘤标志物表达异常,患者血清HE4水平与肿瘤的病理类型及转移情况相关,血清HE4对腺癌有较高的敏感度,血清HE4水平检测可用于肺癌辅助诊断及病情评估。

血清鳞状细胞癌抗原(SCC-Ag)、癌胚抗原(CEA)、细胞角蛋白19片段(CYFRA21-1)和HE4联合检测在宫颈癌诊断中的临床价值

目的以宫颈癌者为对象,探究行HE4(人附睾上皮分泌蛋白4)和CEA(癌胚抗原)、SCC-Ag(血清鳞状细胞癌抗原)和CYFRA21-1(细胞角蛋白19片段)联合检测的效果。方法把2018年1月至2020年12月时段我院接收的100例宫颈癌患者作为疾病组,同期另选取到医院行健康检查者100例作为对照组。实施酶联免疫吸附法与电化学发光法对对象的HE4和CEA、SCC-Ag和CYFRA21-1水平实施检测。结果在比较对象HE4、CEA、SCC-Ag、CYFRA21-1血清水平阳性率中,较疾病组,对照组结果所占比更低(P<0.05)。在比较对象HE4、CEA、SCC-Ag、CYFRA21-1血清水平中,较疾病组,对照组数据评分结果更低(P<0.05)。结论在宫颈癌诊断中,联合检测血清HE4、CEA、SCC-Ag、CYFRA21-1水平中,诊断准确率高,能为后期临床治疗宫颈癌提供依据支持。

抗人氨基末端脂多糖结合蛋白二硫键稳定性Fv抗体的制备及生物学活性的初步研究

目的制备抗人氨基末端脂多糖结合蛋白(N-terminal fragment of human lipopolysaccharide binding protein,NH-LBP)的二硫键稳定性Fv抗体(disulfide stabilized Fv fragment,dsFv),并初步测定其生物学活性。方法将含有dsFv-VL与dsFvVH包涵体蛋白经复性、折叠和纯化,获得完整的dsFv抗体。通过ELISA、TNF-α分泌等方法,初步测定dsFv抗体在体内外的生物学活性。结果获得dsFv抗体蛋白约2.1mg,dsFv与NH-LBP有较好的结合能力,并在动物体内减轻了LPS所诱导的炎症反应,发挥了一定的保护活性。结论通过分别表达VL和VH片段,再制备dsFv抗体是可行的,dsFv能部分抑制LBP的生物学功能。

抗人脂多糖结合蛋白氨基端片段抗体dsFv V_L链的构建、表达和鉴定

目的将抗人脂多糖结合蛋白氨基端片段(NH-LBP)抗体的Fv L链引入半胱氨酸(Cys),并表达、纯化。方法应用mega-primer PCR方法,在抗NH-LBP单克隆Fab抗体的轻链基因骨架区中引入编码Cys的基因序列,将目的序列放入载体pET-28a(+),于工程菌BL21star(DE3)中表达及TALON柱芯亲合纯化,通过ELISA法初步鉴定其与NH-LBP的结合力。结果dsFv VL链的Thr21替换为Cys,扩增出基因片段长约为650bp,经BL21star(DE3)菌表达出相对分子质量约为28×103的目的蛋白,与NH-LBP具有一定的结合力。结论抗体轻链中成功引入了Cys。

人胎儿脑的一个cDNA编码序列及其蛋白质预测

用 m RNA差异显示 PCR技术 ,从人 1 8周、2 2周胎儿脑和肝肾组织的 m RNA逆转录产物得到一些特异性显示的片段 .其中一个随机片段 GC1 0 2作为探针 ,从本实验室构建的 1 8周胎儿脑c DNA基因文库进行杂交筛选 ,得到一个阳性克隆λ gt1 0 /GC1 0 2 .该克隆内插入的 c DNA片段长2 .9kb,经过 DNA测序 ,显示具有一个开放阅读框架 ,编码 1 37个氨基酸的肽链 .用蛋白质结构的建模软件预测了该肽链的立体结构初步模型 .

血清人附睾蛋白4检测在肺癌诊断中的意义

目的探讨人附睾蛋白4（human epididymis protein4，HE4）在肺癌诊断中的意义。方法采用酶联免疫吸附试验检测60例肺癌患者和60例肺良性疾病患者血清中HE4的含量，分析其表达差异；采用电化学发光法检测神经元特异性烯醇化酶（neuron—specific enolase，NSE）、细胞角蛋白19片段（cytokeratin 19 fragment，cyfra21-1）、癌胚抗原（carcinoembryonic antigen，CEA）水平，分析其与HE4表达的相关性。结果HE4在肺癌患者中阳性率（42．0％）低于cyfra21-1（55．0％）、CEA（50．0％），高于NSE（27．0％）。肺癌组HE4水平明显高于肺良性疾病组，差异有统计学意义（P〈0．05），肺癌患者血清HE4水平与NSE、eyfra21—1呈正相关（r=0．478，r=0．300，P均〈0．05），与CEA无相关性（r=0．133．P=0．311）。HE4、NSE、eyfra21-1联合检测可提高肺癌诊断的灵敏度（78．0％）和特异性（86．0％）。结论HE4是有价值的肺癌诊断标志物，与NSE、cyfra21—1联合检测有助于提高肺癌的检出率。

人补体片段C5a蛋白的可溶性表达、纯化及生物学活性检测

目的:为得到可溶性表达的人补体片段C5a蛋白,并检测其生物学活性。方法:用IPTG对C5a融合蛋白进行诱导表达,表达产物经肠激酶酶切后用Ni2+分离柱纯化得到C5a蛋白,通过对中性粒细胞的趋化作用、呼吸爆发、产生乳铁蛋白等实验检测C5a蛋白的生物学活性。结果:成功获得可溶性表达的C5a融合蛋白,通过肠激酶酶切后得到高纯度的C5a蛋白,C5a蛋白对人中性粒细胞具有明显的趋化作用,能引起人中性粒细胞的呼吸爆发并能诱导人中性粒细胞产生乳铁蛋白。结论:可溶性表达了具有生物学活性的人补体片段C5a蛋白,为进一步的临床研究和应用奠定了基础。

DC-CIK细胞免疫治疗联合紫杉醇腹腔灌注化疗对卵巢癌患者HE4、bFGF和CYFRA21-1的影响

目的分析树突状细胞-细胞因子诱导的杀伤细胞(DC-CIK细胞)免疫治疗联合紫杉醇腹腔灌注化疗对卵巢癌患者人附睾蛋白4(HE4)、碱性成纤维细胞生长因子(b FGF)、细胞角蛋白19血清片段21-1(CYFRA21-1)的影响。方法选择2014年1—8月陕西省第二人民医院收治的晚期卵巢癌患者80例,按照抽签法分为常规化疗组(n=50)和免疫治疗组(n=30)。常规化疗组采用紫杉醇常规腹腔灌注化疗;免疫治疗组采用DC-CIK细胞免疫治疗联合紫杉醇腹腔灌注化疗。比较两组患者HE4、b FGF和CYFRA21-1、糖类抗原(CA)19-9、CA125、甲胎蛋白(AFP)水平及不良反应发生情况。结果治疗后,两组患者血清HE4、b FGF和CYFRA21-1、CA19-9、CA125、AFP水平均显著低于治疗前(P<0.01)。治疗后,免疫治疗组患者血清HE4、b FGF和CYFRA21-1、CA19-9、CA125、AFP水平显著低于常规化疗组[(42.3±10.8)pmol/L比(87.9±25.6)pmol/L,(70.3±15.4)ng/L比(91.6±18.5)ng/L,(1.5±0.3)μg/L比(2.4±0.6)μg/L,(14.3±9.8)k U/L比(39.9±10.6)k U/L,(10.8±5.6)k U/L比(38.6±10.5)k U/L,(3.3±1.2)μg/L比(24.7±2.3)μg/L](P<0.01)。两组白细胞减少、贫血、恶心呕吐、肾功能损害、周围神经毒性的发生率比较差异无统计学意义(P>0.05)。结论 DC-CIK细胞免疫治疗联合紫杉醇腹腔灌注化疗可显著降低卵巢癌患者HE4、b FGF和CYFRA21-1水平,且不增加不良反应。

人血清附睾蛋白4及联合癌胚抗原和细胞角蛋白19片段抗原在非小细胞肺癌诊断中的临床价值研究

目的:研究人血清附睾蛋白4(HE4)及联合癌胚抗原(CEA)和细胞角蛋白19片段抗原(CYFRA21-1)在非小细胞肺癌(NSCLC)诊断中的临床价值。方法:选取NSCLC患者88例作为病例组,同期健康体检者70例作为健康对照组,测定血清HE4、CEA和CYFRA21-1浓度,比较两组各肿瘤标志物的表达水平,并用受试者工作特征(ROC)曲线分析各指标单独及联合应用对NSCLC的诊断效能。结果:病例组血清HE4、CEA、CYFRA21-1水平均显著高于健康对照组,差异有统计学意义(P<0.05)。血清HE4、CEA和CYFRA21-1在诊断NSCLC中的ROC曲线下面积(AUC)分别为0.819、0.807和0.774;敏感性分别79.5%、70.5%和54.5%;特异性分别为72.9%、75.7%、94.3%。HE4联合CEA、CYFRA21-1诊断NSCLC的AUC最大(0.875),敏感性为91.4%,特异性为79.9%。血清HE4诊断肺腺癌和肺鳞癌的AUC分别为0.797和0.902;敏感性分别73.8%和91.3%;特异性分别为73.9%、81.4%。结论:HE4对NSCLC有较好的诊断价值,其联合CEA、CYFRA21-1检测有助于提高对NSCLC诊断的价值,并且对肺腺癌和肺鳞癌具有鉴别诊断意义。

人附睾蛋白4和细胞角蛋白19片段联合检测在非小细胞肺癌辅助诊断中的意义

目的探讨人附睾蛋白4(HE4)和细胞角蛋白19片段(CYFRA21-1)联合检测在非小细胞肺癌(NSCLC)辅助诊断中的意义。方法采用电化学发光法分别检测50例NSCLC患者、40例肺炎患者和50名健康体检者血清HE4、CYFRA21-1水平,通过受试者工作特征(ROC)曲线评价2项指标联合检测对NSCLC辅助诊断的价值。结果肺癌患者整体CYFRA21-1、HE4水平及Ⅰ~Ⅱ期肺癌患者HE4水平显著高于肺炎患者及健康体检者(P【0.05)。Ⅲ~Ⅳ期NSCLC患者HE4及CYFRA21-1水平高于Ⅰ~Ⅱ期NSCLC患者(P【0.05)。经ROC曲线分析,HE4和CYFRA21-1联合检测的敏感性显著高于任一单项检测的敏感性。结论血清HE4检测比CYFRA21-1对于NSCLC有更高的早期诊断价值。联合检测HE4和CYFRA21-1对诊断NSCLC有较高的敏感性,适用于临床的肺癌普查。

5种肿瘤标志物联合检测在肺癌诊断中的价值

目的探讨癌胚抗原(CEA)、神经元特异性烯醇化酶(NSE)、细胞角蛋白19片段(Cyfra21-1)、胃泌素释放肽前体(ProGRP)、人附睾蛋白4(HE4)联合检测在肺癌诊断中的价值。方法应用电化学发光法检测240例肺癌患者、70例肺部良性病变患者及120例健康体检者血清CEA、NSE、Cyfra21-1、ProGRP、HE4水平,评估其单独及联合检测在肺癌诊断中的价值。结果肺癌组各肿瘤标志物水平显著高于良性病变组及健康对照组,差异均有统计学意义(P<0.05),良性病变组与健康对照组各肿瘤标志物水平差异无统计学意义(P>0.05)。CEA、NSE、Cyfra21-1、ProGRP、HE4联合检测诊断早期肺癌的曲线下面积(AUC)为0.856,优于各指标单独检测,其敏感度为66.7%,特异度为95.0%;5项指标联合检测诊断晚期肺癌的AUC为0.974,优于各指标单独检测,其敏感度为94.2%,特异度为96.7%。单独检测时,HE4诊断早、晚期肺癌的AUC及敏感度也均高于其他指标。结论CEA、NSE、Cyfra21-1、ProGRP、HE4联合检测可显著提高肺癌诊断敏感度,并有助于早期肺癌的诊断,具有极高的临床推广应用价值。