免疫微阵列同步多元分析系统的建立及其初步应用

本研究建立了一种基于抗体微阵列芯片的用于多个生物样品同步检测的分析方法。通过制备条件实验,确定了抗体在微阵列芯片基片表面的多项固化条件;通过鉴定及应用条件实验,确定了抗体微阵列分析系统用于三种肿瘤蛋白质检测的方法学技术指标。本分析系统体现了微阵列检测的高通量性、夹心免疫分析的高特异性和亲合素-生物素系统的高灵敏度。实验及结果分析表明,该系统具有较强的应用价值及开发潜力。

应用微阵列酶联免疫法检测胃癌患者肿瘤标志物

目的探讨微阵列酶联免疫法(Array-ELISA)检测肿瘤标志物对胃癌的诊断及术后疗效观察上的应用价值。方法采用Array-ELISA同时对28例胃癌术前患者、37例胃癌术后患者(其中10例复发,27例未复发)及60例正常体检者的血清进行6种肿瘤标志物检测。结果胃癌组CA199、CA125、CEA均明显高于正常对照组(P<0.05);胃癌术前组CEA水平明显高于胃癌术后组(P<0.05)。胃癌术后复发组CA199、CEA水平显著高于未复发组(P<0.05)。AFP、PSA、CA153在3组间差异无统计学意义(P>0.05)。CA199、CA125、CEA 3项联合检测,其敏感性为58.5%,特异性为90.0%,准确度为73.6%,与单项指标相比较,敏感性、准确度差异均有统计学意义(P<0.05)。结论 CA199、CA125、CEA 3项指标联合检测可提高胃癌检测的敏感性、准确度;CA199、CEA水平对胃癌术后复发的监测具有一定的参考价值。Array-ELISA检测多种肿瘤标志物可应用于胃癌的诊断及术后疗效观察。

微阵列酶联免疫法检测多项肿瘤标志物诊断结直肠癌的临床价值

目的探讨微阵列酶联免疫法(Array-ELISA)检测多项肿瘤标志物诊断结直肠癌(CRC)的临床价值。方法选择CRC患者49例(CRC组)、结直肠良性疾病患者19例(良性疾病组)、健康体检者71例(对照组),采用Array-ELISA法检测其血清甲胎蛋白(AFP)、癌胚抗原(CEA)、前列腺特异性抗体(PSA)、CA125、CA199、CA153。应用Logistic回归和受试者工作曲线对各指标进行相关性分析。结果 CRC组CA199、CA125、CEA均高于对照组及良性疾病组,良性疾病组CEA高于对照组(P均<0.05);三组CA153、PSA、AFP比较无统计学差异。CA125、CA199、CA153联合检测诊断CRC的敏感性为73.47%、准确度为85.61%、阴性预测值为86.46%,与其单项指标比较均有统计学差异(P均<0.05),其特异性、阳性预测值比较无统计学差异。CA125、CA199、CA153联合检测的曲线下面积大于其单项指标(P<0.05)。结论 CA199、CA125、CEA是CRC的肿瘤相关性标志物,采用Array-ELI技术联合检测三项指标诊断CRC的敏感性、准确度优于其单项指标。

微阵列酶联免疫吸附试验在临床输血检测中的应用

目的探讨微阵列酶联免疫吸附试验(Array-ELISA)的临床应用价值。方法用ELISA和Array-ELISA同时检测150例样本的人类免疫缺陷病毒抗体(抗-HIV)、梅毒螺旋体抗体(抗-TP)和HBsAg,观察对比两种检测方法的结果。结果两种方法对150例样本的检测结果经卡方检验证明差异无统计学意义。除了HBsAg检测结果的总符合率为96.7%,其余指标检测结果的总符合率均为100.0%。结论Array-ELISA与ELISA试剂盒有极高的符合率,初步证明其可以满足临床输血前检测的要求。

基于微阵列化学发光免疫分析系统的血清肿瘤标记物CA72-4参考区间建立

目的:目前,多种血清肿瘤标记物已应用于癌症的诊断、治疗和预后监测。因此,建立合适的肿瘤标记物的参考区间(RI)对于临床医生制定正确的治疗方案非常重要。本研究旨在通过实验室新设立的微阵列化学发光免疫分析系统(MCI)来建立血清糖类抗原72-4 (CA72-4)的参考区间。方法:根据CLSI EP28-A3,选择了相应的统计学分析方法,并基于分析结果采用间接法确定参考区间。研究共选用5937名健康参考个体,通过MCI系统测定的CA72-4血清水平来确定参考区间。这四个研究项目的所有测试数据都呈偏态分布。首先,性别和年龄是影响检测价值水平的两个重要因素。其次,按性别和年龄对数据进行分组,使用非参数排序法建立每个组的参考区间。结果:血清CA72-4水平总体呈偏态分布,不同性别、年龄组的血清CA72-4水平无统计学意义。因此,可以通过非参数排序法,按照95%置信区间计算出健康个体的CA72-4参考区间是0~13.34 U/mL。结论:新建立的参考区间更适合国内研发的MCI系统,对于临床医学诊断和治疗管理决策更有价值。

6项肿瘤标志物应用微阵列酶联免疫法与电化学发光免疫分析法测定的对比研究

目的对比微阵列酶联免疫法(Array-ELISA)与电化学发光免疫分析法(ECLIA)测定6项肿瘤标志物的效果。方法选择2018年4月—2019年4月该院收治的202例肿瘤患者作为研究对象。通过Array-ELISA法与ECLIA法检测6项肿瘤标志物,即甲胎蛋白(AFP)、癌胚抗原(CEA)、糖类抗原199(CA199)、糖类抗原125(CA125)、前列腺特异性抗原(PSA)、和糖类抗原153 (CA153)。结果 ECLIA法对于CA199与CA153诊断的阳性率82.76%、78.13%高于Array-ELISA法的55.17%、53.13%,差异有统计学意义(χ~2=5.156、4.433,P<0.05)。通过Spearman检测,Array-ELISA法与ECLIA法对6项肿瘤标志物的检测具有正相关性(r=0.685~0.957,P<0.01)。Array-ELISA法与ECLIA法对CEA、AFP、CA199、CA125、PSA与相应疾病类型的ROC曲线面积具有一致性(ROC曲线下面积介于0.615~0.978之间)。Array-ELISA法检测CA153的ROC曲线面积(0.680)低于ECLIA法(0.842)。结论 ArrayELISA法与ECLIA法对于6项肿瘤标志物检测具有较佳的一致性,鉴于ECLIA试剂成本过高,临床可引入Array-ELISA对常规人群进行筛查与体检。

微阵列酶联免疫技术检测糖尿病自身抗体的临床应用

目的探讨微阵列酶联免疫技术(Array-ELISA)用于检测糖尿病自身抗体的临床应用价值。方法选择2020年6—12月在广东省中医院就诊的120例糖尿病患者作为研究对象,其中1型糖尿病(T1DM)患者72例作为T1DM组,2型糖尿病(T2DM)患者48例作为T2DM组;另外选择同期23名健康体检者作为正常对照组。采用Array-ELISA作为试验方法,条带免疫印迹法(IBT)作为对比方法,检测各组谷氨酸脱羧酶抗体(GADA)、酪氨酸磷酸酶抗体(IA-2A)、胰岛细胞抗体(ICA)、锌转运体8抗体(ZnT8A)和胰岛素抗体(IAA)5种抗体,评价两种方法的一致性;分析Array-ELISA检测各组5种抗体的阳性率,比较单独和同时检测5种抗体的诊断效能。结果Array-ELISA和IBT两种方法检测GADA、IA-2A、ICA、ZnT8A和IAA的总符合率均大于95.00%(GADA为98.60%,IA-2A为98.60%,ICA为97.20%,ZnT8A为97.20%,IAA为95.80%),Kappa值均大于0.75(GADA为0.95,IA-2A为0.93,ICA为0.88,ZnT8A为0.86,IAA为0.85),配对χ2检验的P值均大于0.05(GADA为0.50,IA-2A为0.50,ICA为0.13,ZnT8A为0.63,IAA为0.69),两种检测方法具有高度一致性。Array-ELISA检测T1DM患者5种抗体的阳性率均明显高于T2DM组和正常对照组〔GADA为34.72%(25/72)比0.00%(0/23)、0.00%(0/48),IA-2A为20.83%(15/72)比0.00%(0/23)、2.08%(1/48),ICA为30.56%(22/72)比0.00%(0/23)、0.00%(0/48),ZnT8A为20.83%(15/72)比0.00%(0/23)、0.00%(0/48),IAA为31.94%(23/72)比0.00%(0/23)、2.08%(1/48),均P<0.05〕。Array-ELISA同时检测T1DM组5种抗体的敏感度为58.33%,特异度为97.18%,诊断符合率为77.62%。结论Array-ELISA作为一种新方法同时检测5种糖尿病自身抗体对糖尿病的诊断分型具有一定的临床应用价值。

微阵列ELFA和IBT 2种过敏原筛查方法临床应用评价

目的比较微阵列酶联免疫荧光法(ELFA)和免疫印迹法(IBT)在过敏原筛查中的差异。方法选取225例于上海中医药大学附属龙华医院皮肤科就诊患者,采用IBT和微阵列ELFA进行吸入性及食物性过敏原特异性IgE(s IgE)检测。结果在225例患者中,IBT阳性51例,阳性率为22.7%,抗原阳性率从高到低位于前4位的依次为屋尘螨/粉尘螨、鳕鱼/龙虾/扇贝、屋尘、猫毛;微阵列ELFA阳性82例,阳性率为36.4%,抗原阳性率从高到低位于前4位的依次为螨虫组合(粉尘螨/屋尘螨/热带无爪螨)、蟑螂组合(德国蟑螂/亚洲蟑螂)、蟹、猫毛。2种方法对尘螨、蟑螂、猫毛、海鱼组合、蟹的分级一致性Kappa值分别为38.2%、6.04%、32.1%、22.2%、13.4%。结论微阵列ELFA与IBT在临床检测中有较大差异,微阵列ELFA包含更多的过敏原,具有更高的阳性率,2种方法应互为补充以提高阳性率。

具有3D微纳结构PDMS阵列免疫传感芯片研制

介绍了一种简便快速加工微阵列免疫传感芯片的新方法。采用化学刻蚀技术加工具有μm级山脉状起伏和nm级表面粗糙度结构(简称为3D微纳表面)的玻璃阳模,以该阳模为模板浇注法制得表面具有3D微纳表面结构的PDMS基片,再借助于物理吸附,将抗体直接固定于该PDMS表面,形成具有3D微纳结构的PDMS微阵列免疫传感器。利用光学显微镜和原子力显微镜对玻璃阳模和PDMS基片表面形貌进行表征,研究了PDMS表面微纳结构化处理对抗体吸附能力的影响。结果表明:3D微纳结构的PDMS由于具有大的比表面积,能显著增强抗体的吸附能力。将研制所得的3D微纳表面结构的PDMS芯片用于微阵列荧光免疫分析,其灵敏度是平板PDMS的5倍。

探讨微阵列酶联免疫法在艾滋病哨点监测工作中的应用

目的:探讨微阵列酶联免疫法检测的临床价值。方法:用酶联免疫吸附试验(ELISA)和微阵列酶联免疫法(Ar-ray-ELISA)检测试验组样本的抗-HIV抗体、抗-TP抗体。分别统计两种方法检测阳性、阴性的样本数目,并进行统计学处理。结果:两种方法分别检测400份实验组样本,统计检测结果并经卡方检验证明无差别。检测结果的总符合率均为100%。结论:微阵列酶联免疫法与ELISA法无统计学差异,初步证明可以满足艾滋病哨点监测工作中检测工作的要求。

微阵列酶联免疫法在临床输血检测中的应用

目的:探讨微阵列酶联免疫法检测的临床价值。方法:用酶联免疫法(ELISA)和微阵列酶联免疫法检测对照组样本的抗-HIV抗体、抗-TP抗体、HBsAg。分别统计2种方法检测阳性、阴性的样本数目,并进行统计学处理。结果:2种方法分别检测140份实验组样本,统计检测结果并经卡方检验证明差异无统计学意义。除了HBsAg检测结果的总符合率为98.6%,其余指标检测结果的总符合率均为100%。结论:微阵列酶联免疫法与ELISA法差异无统计学意义,初步证明可以满足临床输血检测的要求。

肿瘤标志物联合检测在乳腺癌诊断中的价值

目的探讨微阵列酶联免疫法(Array-ELISA)检测肿瘤标志物诊断乳腺癌的价值。方法采用Array-ELISA对146例乳腺癌患者、64例乳腺良性疾病患者及119例健康体检者的血清进行甲胎蛋白(AFP)、癌胚抗原(CEA)、癌抗原125(CA125)、癌抗原153(CA153)、糖链抗原199(CA199)、前列腺特异抗原(PSA)6种肿瘤标志物检测。应用Logistic回归和ROC曲线对各指标进行分析。结果乳腺癌组CA153、CA125均明显高于乳腺良性疾病组与正常对照组(P<0.05);其他四种肿瘤标志物(AFP、PSA、CA199、CEA)在3组间差异无统计学意义(P>0.05)。CA153、CA125两项联合检测,其敏感性为81.51%、准确度为86.93%、阴性预测值为86.08%,与单项指标比较差异均有统计学意义(P<0.05)。CA153、CA125两项肿瘤标志物单独检测时,CA153的AUC为0.874较CA125大;两项联合指标的AUC达0.913,大于各单项肿瘤标志物(P<0.05)。结论 CA153、CA125是乳腺癌的肿瘤相关性标志物,CA153对于乳腺癌的诊断价值更大。2项指标联合检测优于单一的肿瘤标志物,可提高诊断乳腺癌的正确性。Array-ELISA检测多种肿瘤标志物可应用于乳腺癌的诊断。

Array-ELISA法和ECLIA法测定六项肿瘤标志物的比较研究

目的分析和评价6项肿瘤标志物测定试剂盒[微阵列酶联免疫法(Array-ELISA)]在肿瘤标志物检测中的应用价值。方法采用Array-ELISA和电化学发光免疫分析法(ECLIA)检测相同标本的6项临床常见肿瘤标志物:甲胎蛋白(AFP)、癌胚抗原(CEA)、前列腺特异性抗原(PSA)、糖类抗原125(CA125)、糖类抗原199(CA199)和糖类抗原153(CA153)。采用受试者工作特征(ROC)曲线进行分析。结果 2种方法检测AFP、CEA、PSA和CA125的阳性率差异无统计学意义(P>0.05),检测CA199和CA153的阳性率差异有统计学意义(P<0.01)。2种方法对AFP、CEA、PSA、CA125和CA199的检测结果总符合率均>85%,仅CA153的总符合率为61.1%。2种方法对6项肿瘤标志物的检测结果显著相关(P<0.01),相关系数(r)为0.695～0.960。2种方法检测AFP、CEA、PSA、CA125和CA199对相关肿瘤诊断的ROC曲线下面积介于0.62～0.99之间;用Array-ELISA检测CA153对乳腺癌诊断的ROC曲线下面积低于ECLIA。结论 Array-ELISA与ECLIA对6项肿瘤标志物的检测结果均有良好一致性,可以引入Array-ELISA检测6项肿瘤标志物作为常规体检项目和筛查项目。

TORCH感染孕妇IgG亲和力检测的临床价值

目的通过检测TORCH感染孕妇IgG亲和力指数(AI),探讨TORCH感染类型与妊娠结局间关系。方法收集TORCH各型病原体IgM阳性孕妇血清,检测其IgG亲和力指数(AI),并追踪妊娠结局。结果在TORCH各病原体近期感染的孕妇中,HSV(含1型及2型)、RUB、CMV、TOXO原发感染(AI<30%)的比例分别为0、3.8%、9.3%、7.9%;在CMV原发感染的10例孕妇中,2例妊娠结局异常(稽留流产),CMV疑似原发感染孕妇中发现1例为异常妊娠;TOXO原发感染孕妇发现1例为胎儿畸形(脑积水),其余均为正常妊娠。结论在TORCH各病原体近期感染的孕妇中,以非原发性感染为主;而巨细胞及弓形虫原发感染对胎儿的侵害则远大于非原发感染。

RNA结合蛋白与RNA相互作用鉴定技术

RNA结合蛋白(RNA binding proteins,RBPs)通过与RNA相互作用,广泛参与到RNA的剪切、转运、编辑、胞内定位及翻译调控等过程中。RNA领域尤其是非编码RNA(non-coding RNA,ncRNA)研究的快速发展,催生了多种RBPs-RNAs相互作用鉴定技术。这些技术反之又推动了RNA领域的研究进程。本文对紫外交联免疫沉淀(ultraviolet crosslinking and immunoprecipitation,CLIP),CLIP cDNA文库高通量测序(high-throughput sequencing of CLIP cDNA library,HITS-CLIP),光活化核苷增强的CLIP(photoactivatable-ribonucleoside-enhanced crosslinking and immunoprecipitation,PAR-CLIP),单核苷酸分离CLIP(individual nucleotide resolution CLIP,i CLIP),TRIBE(targets of RNA-binding protein identified by editing),RNA标记,相互作用组捕获(interactome capture,IC)和Ser IC(serial RNA interactome capture)等RBPs-RNAs相互作用鉴定技术的基本原理和优缺点以及应用进行综述。

多项肿瘤标记物在胃癌诊断中的筛选及应用价值

目的探讨多项肿瘤标记物在胃癌诊断中的筛选及应用价值。方法通过Array-ELISA检测胃癌患者(胃癌组)、健康体检者(对照组)血清中在癌胚抗原(CEA)、糖类抗原199(CA199)、糖类抗原242(CA242)、糖类抗原724(CA724)、糖类抗原50(CA50)、甲胎蛋白(AFP)、糖类抗原125(CA125)、糖类抗原153(CA153)、人绒毛膜促性腺激素(HCG)、糖分解烯醇酶(NSE)这10种肿瘤标志物的水平,并考察这些单项肿瘤标志物与多项联合检测胃癌的敏感度、特异度和准确度。结果胃癌组除HCG之外,其余9种肿瘤标志物水平较对照组均明显升高(P<0.05)。单项检测灵敏度、特异度及准确度最高的前三位肿瘤标记物,共计4种,分别为CA724、CA199、CEA及AFP。CA724+CA199+CEA+AFP四联联合检测的灵敏度、特异度及准确度最高,分别为96.50%、97.94%、91.11%。结论采用Array-ELISA联合检测CA724、CA199、CEA及AFP将大大提升胃癌的早期诊断水平。

Survey of molecular profiling during human colon cancer development and progression by immunohistochemical staining on tissue microarray

AIM： To explore the molecular events taking place during human colon cancer development and progression through high-throughput tissue microarray analysis. METHODS： We constructed two separate tissue microarrays containing 1.0 mm or 1.5 mm cylindrical samples acquired from 112 formalin-fixed and paraffinembedded blocks, including carcinomas （n = 85）, adenomatous polyps （n = 18）, as well as normal paracancerous colon tissues （n = 9）. Immunohistochemical staining was applied to the analysis of the consecutive tissue microarray sections with antibodies for 11 different proteins, including p53, p21, bcl-2, bax, cyclin D1, PTEN, p-Aktl, β-catenin, c-myc, nm23-h1 and Cox-2. RESULTS： The protein expressions of p53, bcl-2, bax, cyclin D1, β-catenin, c-myc, Cox-2 and nm23-h1 varied significantly among tissues from cancer, adenomatous polyps and normal colon mucosa （P = 0.003, P = 0.001, P = 0.000, P = 0.000, P = 0.034, P = 0.003, P = 0.002, and P = 0.007, respectively）. Chi-square analysis showed that the statistically significant variables were p53, p21, bax, β-catenin, c-myc, PTEN, p-Aktl, Cox-2 and nm23-h1 for histological grade （P = 0.005, P = 0.013, P = 0.044, P = 0.000, P = 0.000, P = 0.029, P = 0.000, P = 0.008, and P = 0.000, respectively）, β-catenin, comyc and p-Akt1 for lymph node metastasis （P = 0.011, P =0.005, and P = 0.032, respectively）, β-catenin, c-myc, Cox-2 and nm23-h1 for distance metastasis （P = 0.020, P = 0.000, P = 0.026, and P = 0.008, respectively）, and cyclin D1, β-catenin, c-myc, Cox-2 and nm23h1 for clinical stages （P = 0.038, P = 0.008, P = 0.000, P = 0.016, and P = 0.014, respectively）. CONCLUSION： Tissue microarray immunohistochemical staining enables high-throughput analysis of genetic alterations contributing to human colon cancer development and progression. Our results implicate the potential roles of p53, cyclin D1, bcl-2, bax, Cox-2, β-catenin and c-myc in development of human colon cancer and that of bcl-2, nm23-h1, PTEN and p-Akt1 in progression of human colon cancer.

Reliability of a Tissue Microarray in Detecting Thyroid Transcription Factor-1 Protein in Lung Carcinomas

OBJECTIVE To compare the expression of the thyroid transcription factor-1 （TTF-1） in human normal adult type Ⅱ alveolar epithelial cells, embryonic pneumocytes and cancer cells of lung carcinoma and metastatic lymph nodes using a tissue microarray （TMA） along with paired conventional full sections, and to investigate the reliability of tissue microarrays in detecting protein expression in lung carcinoma. METHODS A lung carcinoma TMA including 765 cores was constructed. TTF-1 protein expression in both TMA and paired conventional full sections were detected by the immunohistochemical SP method using a monoclonal antibody to TTF-1. A PU （Positive Unit） of TTF-1 protein was assessed quantitatively by the Leica Q500MC image analysis system with results from the paired conventional full sections as controls. RESULTS There was no significance between TMA and paired conventional full sections in TTF-1 expression in different nuclei of the lung tissue. CONCLUSION TTF-1 protein expression in lung carcinoma detected by TMA was highly concordant with that of paired full sections. TMA is a reliable method in detecting protein expression.

Gene expression profiling and endothelin in acute experimental pancreatitis

AIM:To analyze gene expression profiles in an experimental pancreatitis and provide functional reversal of hypersensitivity with candidate gene endothelin-1 antagonists.METHODS:Dibutyltin dichloride(DBTC) is a chemical used as a polyvinyl carbonate stabilizer/catalyzer,biocide in agriculture,antifouling agent in paint and fabric.DBTC induces an acute pancreatitis flare through generation of reactive oxygen species.Lewis-inbred rats received a single i.v.injection with either DBTC or vehicle.Spinal cord and dorsal root ganglia(DRG) were taken at the peak of inflammation and processed for transcriptional profiling with a cDNA microarray biased for rat brain-specific genes.In a second study,groups of animals with DBTC-induced pancreatitis were treated with endothelin(ET) receptor antagonists [ET-A(BQ123) and ET-B BQ788)].Spontaneous pain related mechanical and thermal hypersensitivity were measured.Immunohistochemical analysis was performed using anti-ET-A and ET-B antibodies on sections from pancreatic tissues and DRG of the T10-12 spinal segments.RESULTS:Animals developed acute pancreatic inflammation persisting 7-10 d as confirmed by pathological studies(edema in parenchyma,loss of pancreatic architecture and islets,infiltration of inflammatory cells,neutrophil and mononuclear cells,degeneration,vacuolization and necrosis of acinar cells) and the painrelated behaviors(cutaneous secondary mechanical and thermal hypersensitivity).Gene expression profile was different in the spinal cord from animals with pancreatitis compared to the vehicle control group.Over 260 up-regulated and 60 down-regulated unique genes could be classified into 8 functional gene families:circulatory/acute phase/immunomodulatory;extracellular matrix;structural;channel/receptor/transporter;signaling transduction;transcription/translation-related;antioxidants/chaperones/heat shock;pancreatic and other enzymes.ET-1 was among the 52 candidate genes upregulated greater than 2-fold in animals with pancreatic inflammation and visceral pain-related behavior.Treatments with the ET-A(BQ123) and ET-B(BQ-788) antagonists revealed significant protection against inflammatory pain related mechanical and thermal hypersensitivity behaviors in animals with pancreatitis(P < 0.05).Open field spontaneous behavioral activity(at baseline,day 6 and 30 min after drug treatments(BQ123,BQ788) showed overall stable activity levels indicating that the drugs produced no undesirable effects on normal exploratory behaviors,except for a trend toward reduction of the active time and increase in resting time at the highest dose(300 μmol/L).Immunocytochemical localization revealed that expression of ET-A and ET-B receptors increased in DRG from animals with pancreatitis.Endothelin receptor localization was combined in dual staining with neuronal marker NeuN,and glia marker,glial fibrillary acidic protein.ET-A was expressed in the cell bodies and occasional nuclei of DRG neurons in na ve animals.However,phenotypic expression of ET-A receptor was greatly increased in neurons of all sizes in animals with pancreatitis.Similarly,ET-B receptor was localized in neurons and in the satellite glia,as well as in the Schwann cell glial myelin sheaths surrounding the axons passing through the DRG.CONCLUSION:Endothelin-receptor antagonists protect against inflammatory pain responses without interfering with normal exploratory behaviors.Candidate genes can serve as future biomarkers for diagnosis and/or targeted gene therapy.