肺炎支原体肺炎患儿血清MICA、OPN水平及其与反复呼吸道感染的相关性研究

目的探究肺炎支原体肺炎患儿血清主要组织相容性复合物Ⅰ链相关基因A(MICA)、骨桥蛋白(OPN)水平及其与反复呼吸道感染的相关性。方法选取该院2019年3月至2021年3月收治的肺炎支原体肺炎患儿106例作为研究组,另选取同期于该院进行体检的健康儿童106例作为对照组,根据肺炎支原体肺炎患儿是否发生反复呼吸道感染分为反复呼吸道感染发生组和反复呼吸道感染未发生组;使用全自动微生物鉴定系统和纸片扩散试纸进行病原菌检测以及耐药性试验;血清MICA、OPN水平检测采用酶联免疫吸附试验;采用多因素Logistic回归分析影响肺炎支原体肺炎反复呼吸道感染发生的危险因素;绘制受试者工作特征(ROC)曲线分析血清MICA、OPN单独及联合检测对肺炎支原体肺炎患儿发生反复呼吸道感染的预测价值。结果106例肺炎支原体肺炎患儿共分离出116株菌株,其中革兰阴性菌77株(66.38%),包括流感嗜血杆菌29株(25.00%),肺炎克雷伯菌17株(14.66%),鲍曼不动杆菌14株(12.07%),铜绿假单胞菌8株(6.90%),阴沟肠杆菌6株(5.17%),其他菌3株(2.59%);革兰阳性菌39株(33.62%),包括金黄色葡萄球菌16株(13.79%),表皮葡萄球菌10株(8.62%),肠球菌6株(5.17%),溶血葡萄球菌5株(4.31%),其他菌2株(1.72%)。流感嗜血杆菌耐药率较高的为头孢哌酮,占75.86%,肺炎克雷伯菌耐药率较高的为氨苄西林,占88.24%。16株金黄色葡萄球菌中,对红霉素耐药12株(75.00%),对环丙沙星耐药8株(50.00%),对四环素耐药6株(37.50%),对苯唑西林耐药4株(25.00%),对克林霉素耐药2株(12.50%),未发现对万古霉素和利奈唑胺耐药的金黄色葡萄球菌。研究组血清MICA、OPN水平均明显高于对照组,差异均有统计学意义(P<0.05)。46例患儿发生反复呼吸道感染,60例患儿未发生反复呼吸道感染。反复呼吸道感染发生组使用药物不当比例,血清MICA、OPN水平均明显高于反复呼吸道感染未发生组,差异均有统计学意义(P<0.05)。多因素Logistic回归分析结果显示,MICA水平升高(95%CI:1.782~3.949)、OPN水平升高(95%CI:1.989~5.012)均为肺炎支原体肺炎发生反复呼吸道感染的危险因素(P<0.05)。ROC曲线分析结果显示,血清MICA预测肺炎支原体肺炎反复呼吸道感染的曲线下面积(AUC)为0.899(95%CI:0.836~0.962),截断值为153.702 pg/mL,灵敏度为76.51%,特异度为87.24%。血清OPN预测肺炎支原体肺炎反复呼吸道感染的AUC为0.898(95%CI:0.835~0.960),截断值为101.231 pg/mL,灵敏度为78.29%,特异度为84.41%。二者联合检测预测肺炎支原体肺炎反复呼吸道感染的AUC为0.954(95%CI:0.918~0.989),灵敏度为88.35%,特异度为80.24%。二者联合检测预测肺炎支原体肺炎患儿发生反复呼吸道感染的AUC优于血清MICA、OPN各自单独预测的AUC(Z_(联合vs.MICA)=2.624、Z_(联合vs.OPN)=2.735,P<0.05)。结论肺炎支原体肺炎患儿血清MICA、OPN水平明显升高,二者与反复呼吸道感染密切相关。

Anti-human leukocyte antigens and anti-major histocompatibility complex class I-related chain A antibody expression in kidney transplantation during a four-year follow-up

Background Humoral immunity is an important factor for long-term survival of renal allograft. Here we performed a four-year follow-up to explore the clinical significance of monitoring anti-human leukocyte antigens （HLA） and anti-major histocompatibility complex class I-related chain A （MICA） antibody expression after kidney transplantation. Methods We obtained serial serum samples from 84 kidney transplant patients over a four-year period. All patients were followed up at least 6 months after transplantation and had at least two follow-up points. Anti-HLA and anti-MICA antibody titres and serum creatinine （SCr） levels were evaluated at each follow-up. Patients were divided into 4 groups： HLA（＋） MICA（-）, HLA（-）MICA（＋）, HLA（＋）MICA（＋） and HLA（-）MICA（-）. The impact of post-transplant antibody level on kidney allograft function was evaluated. Results Antibodies were detected in 38.1% （32/84） of the renal allograft recipients. HLA, MICA and HLA＋MICA expression was observed in 18.89%, 14.44% and 5.93% of the recipients respectively. The most frequent anti-HLA and anti-MICA specific antibodies identified were All, A24, A29, A32, A33, A80; B7, B13, B37; DR17, DR12, DR18, DR52, DR53, DR1, DR4, DR9, DR51; DQ7, DQ4, DQ8, DQ2, DQ9, DQ5, DQ6 and MICA02, MICA18, MICA19, MICA07, MICA27. As the time after transplantation elapsed, more recipients developed de novo antibody expression. Total 11.91% （10/84） of the recipients had de novo antibody expression during the follow up. The average level of SCr and the percentage of recipients with abnormal allograft function were significantly higher in recipients with anti-HLA and/or anti- MICA antibody expression than those without. The appearance of anti-HLA and anti-MICA antibody expression always preceded the increase in SCr value. Conclusions Anti-HLA and anti-MICA antibody expression has predictive value for early and late allograft dysfunction. The presence of donor specific antibody is detrimental to graft function and graft survival.

Serum major-histocompatibility-complex class Ⅰ-related chain A antibody detection for the evaluation of graft dysfunction in renal allograft recipients

Background In addition to the well-known antibodies against human leukocyte antigens （HLA）-induced kidney-graft rejection, polymorphic major-histocompatibility-complex （MHC） class Ⅰ-related chain A （MICA） antigens can elicit antibodies and have been suggested to play a role in the antibody-mediated allograft rejection （AMR）. We carded out a prospective study of MICA antibodies in post-renal transplant patients to determine the association between MICA antibodies, C4d staining, histological features, and graft outcome.Methods We tested 52 patients who had biopsy results due to graft dysfunction. The MICA antibodies in concurrent sera were determined by Luminex. All patients were followed up for one year after renal biopsy. The influence of antibody production on the function of graft was analyzed.Results Antibodies against MICA were positive in 15 out of the 52 patients （28.9%）. The presence of MICA antibodies was associated with renal-allograft deterioration. During one-year follow-up, the estimated glomerular filtration rate （eGFR） decreased （24.0±3.4）% among recipients with anti-MICA antibodies. However, among recipients without anti-MICA antibodies, the eGFR has declined only （8.4＋3.0）% （P=0.017）. The association between C4d staining,histological features and MICA antibody production was found no significant difference.Conclusion Besides anti-HLA antibodies, the presence of post-transplant MICA antibody is associated with poor graft outcome and increases the risk of graft failure.

Antibodies against major histocompatibility complex class I-related chain A in transplant recipients

Objective To review the role of polymorphism of major histocompatibility complex class I-related chain A （MICA） gene and antibodies against MICA antigens in transplant immunology. Data sources The data used in this review were mainly from our own results and from the relevant English language literatures published from 1999 to 2010. Some data presented in this review are in press.Study selection Articles regarding MICA gene discovery and pioneering finding of antibodies against MICA antigen and allograft rejection were selected. This review chronicles the development of our understanding of the role that MICA antigens and antibodies may play in organ transplantation.Results Polymorphic glycoprotein MICA antigens were detected on freshly isolated human umbilical cord endothelial cells, but not on peripheral lymphocytes. Antibodies were found and typing of recipients and donors by sequencing the MICA alleles has established that de novo antibodies produced in kidney transplant recipients are directed at mismatched MICA epitopes and are associated with acute rejection and chronic transplant failure. The specificity of antibodies against the epitopes of MICA antigens were well characterized by donor MICA typing, single antigen array testing with antibody absorption and elution. Acute graft-versus-host disease was observed in stem-cell recipients who were mismatched for MICA.Conclusions Immunization against mismatched MICA epitopes encountered in donor organs after transplantation may result in antibodies against MICA alleles. Testing for MICA donor-specific antibodies （DSA） which are associated with early failure of kidney transplants may be helpful for identifying some of the targets of antibodies against antigens other than the human leukocyte antigen （HLA） and for improving transplantation outcome.

Expression characteristics of major histocompatibility complex class I-related chain A antibodies and immunoadsorption effect in sensitized recipients of kidney transplantation

Background Sensitized recipients have a high risk of immunological graft loss due to hyperacute rejection and/or accelerated acute rejection. The presence of major histocompatibility complex class I-related chain A （MICA） antibodies has also been described associated with an increased rate of kidney-allograft rejection. The aim of this study was to describe the expression of MICA antibodies in sensitized recipients of renal transplantation and evaluate its influence on the kidney transplantation recipients.Methods A total of 29 sensitized recipients were included in this study. All patients received the MICA antibodies detection before and after protein A immunoadsorption. Panel reactive antibody （PRA）, HLA-matches, acute rejection and postoperative one to four-week serum creatinine level were also collected and analyzed, respectively. No prisoners were used in this study.Results Eight patients （27.6%） in all 29 sensitized recipients expressed the MICA antibodies but did not show higher acute rejection rate than the non-expressed patients （3/8, 37.5% vs. 8/21, 38.1%; P=1.000）. Recipients with PRA 〉40% showed higher expression levels of MICA antibodies than the recipients with PRA 〈40% （7/16, 43.8% vs. 1/13, 8.3%; P=0.044）. HLA mismatch did not have any effect on the expression of MICA antibodies （P=1.000）. MICA antibodies positive group had higher serum creatinine level than the control in postoperative one week （（135.4±21.4） μmol/L vs. （108.6±31.6） μmol/L, P=0.036）, but no significant difference in postoperative four weeks （（89.0±17.1） μmol/L vs. （77.1±15.9） μmol/L, P=0.089）. MICA antibodies decreased significantly after protein A immunoadsorption.Conclusions MICA antibodies increase in the sensitized recipients, which have significant effects on the function of aliograft in early postoperative period. Protein A immunoadsorption can decrease MICA antibodies effectively in sensitized recipients.

低表达MICA/MICB导致NK细胞对人鼻咽癌多药耐药细胞(CNE2/DDP)杀伤活性下降

目的探讨HLAⅠ类分子及MHCⅠ类链相关分子(MICA/MICB)在人鼻咽癌细胞株CNE2及多药耐药细胞株CNE2/DDP的表达及其对NK细胞杀伤活性的影响。方法流式细胞仪检测CNE2和CNE2/DDP细胞表面HLAⅠ类分子和MICA/MICB的表达情况;LDH释放法测定3例健康者的NK细胞在不同效靶比时对CNE2、CNE2/DDP细胞的杀伤活性;效靶比10∶1时,用抗HLAⅠ类分子单抗(W6/32)和抗MICA/MICB单抗(BAMO-1)分别封闭HLAⅠ类分子和MICA/MICB,观察NK细胞杀伤CNE2、CNE2/DDP细胞活性的变化。结果CNE2/DDP细胞表面HLAⅠ类分子和MICA/MICB的表达均较CNE2细胞明显减少(P<0.01)。NK细胞对CNE2、CNE2/DDP细胞的杀伤活性在效靶比5∶1时分别是(9.37±2.14)%、(4.37±0·63)%;效靶比10∶1时分别是(27.14±1.82)%、(15.79±2.87)%;效靶比20∶1时分别是(36.40±4.28)%、(26.20±4·18)%;效靶比301时分别是(54.67±2.80)%、(40.29±2.73)%。各效靶比时NK细胞对CNE2、CNE2/DDP细胞的杀伤活性与HLAⅠ类分子和MICA/MICB相关,NK细胞对CNE2/DDP细胞的杀伤活性明显低于CNE2细胞(P<0.01)。效靶比10∶1时,W6/32明显增强NK细胞对CNE2、CNE2/DDP细胞的杀伤活性(P<0.01),BAMO-1明显抑制NK细胞对CNE2、CNE2/DDP细胞的杀伤活性(P<0.01)。结论HLAⅠ类分子和MICA/MICB在CNE2、CNE2/DDP的表达差异影响着NK细胞的杀伤活性,MICA/MICB在多药耐药肿瘤细胞的低表达导致耐药肿瘤细胞对NK细胞杀伤敏感性下降。

湖北省汉族人群MICA基因外显子2～4的多态性分析

目的了解湖北省汉族正常人群中MICA等位基因的分布，为研究MICA基因与疾病的关系提供实验基础。方法采用PCR-SSP方法对193例湖北地区汉族正常人群MICA基因外显子2-4的多态性进行分析。结果MICA各等位基因分布频率存在差异，其中以MICA＊00801／02等位基因频率最高（33．7％），其次为MICA＊010（18．4％）、MICA＊00201／020（13．9％）和MICA＊01201／02（9．6％），频率最低的是MICA＊005（0．5％）和MICA＊027（0．5％）。结论湖北地区汉族人群MICA等位基因的构成与其他人群之间存在差异，有自己的分布特征。

抗-MICA抗体在ESRD患者中的表达及其临床意义

目的探讨主要组织相容性复合物I类相关链A(MICA)抗体在终末期肾脏疾病(ESRD)患者中的表达。方法采用液相芯片分析技术和带有11种MICA抗原的荧光微球,对110例ESRD患者进行抗-MICA抗体的检测和抗-MICA抗体的特异性分析。结果在30例PRA阳性患者中抗-MICA抗体(+)的几率为40%(12/30),在80例PRA阴性患者中抗-MICA抗体(+)的几率为17.5%(14/80)。PRA阳性组患者与PRA阴性组患者抗-MICA抗体(+)几率之间呈显著性差异(χ2=6.120,P=0.013)。调查发现,26例MICA抗体(+)血清中表达出11种MICA抗原中的10种抗-MICA抗体特异性,其中,26.92%(7/26)为单特异性抗体,73.08%(19/26)为多特异性抗体。在随后的临床研究中还观察到,3例抗-MICA抗体(+)的患者接受尸体肾移植,术后随访2月,没有发生急性排斥并且移植肾功能良好。结论在PRA阳性患者中抗-MICA抗体(+)的几率亦高,说明抗-MICA抗体(+)的几率与PRA阳性的几率有明显的伴随关联。抗-MICA抗体表现为多特异性,抗-MICA抗体可能包含有IgM和IgG两种免疫球蛋白类型。研究提示,对于这部分ESRD患者未来接受移植替代治疗时,本研究数据将可以作为前瞻性数据提供临床进一步研究MICA与肾移植的关联和影响。

人类MICA基因多态与氯氮平致白细胞减少症的关联分析

目的探讨M ICA基因第5外显子微卫星多态性与氯氮平诱发的白细胞减少症的关联性。方法应用聚合酶链反应和片段长度多态性分析,对93例健康对照者和72例氯氮平(或氯丙嗪)诱发白细胞减少者作M ICA基因第5外显子的多态性研究。结果(1)发现M ICA第5外显子的5种等位基因,并确定了在病例组和健康对照组中的分布频率。(2)表明M ICA第5外显子的A5和A5.1等位基因与精神药物诱发白细胞减少症有关联。(3)M ICA基因的等位基因和基因型分布在氯氮平诱发白细胞减少者与健康对照者之间无差异,但是在氯氮平诱发白细胞减少者与服非氯氮平者之间有显著差异。(4)氯氮平诱发白细胞减少与M ICA第5外显子的A5(OR=0.36,P<0.05,95%C I=0.86-0.15)和A5.1(OR=6.47,P<0.05,95%C I=31.50-1.33)相关联。结论M ICA基因的等位基因A5.1可能是氯氮平诱发白细胞减少症的风险因子,但是对于氯氮平不是专一的。

MICA多态性与白血病易感性的关联研究

目的采用直接测序法对主要组织相容性复合物Ⅰ类链相关A基因(major histocompatibility complex classichain-related A,MICA)进行分型,了解MICA等位基因在正常人群、急性淋巴细胞白血病(acute lymphocytic leukemia,ALL)、急性髓性白血病(acute myeloid leukemia,AML)、骨髓增生异常综合征(myelodysplastic syndrome,MDS)患者中分布的差异。方法选取2016年北京市红十字血液中心167份白血病患者DNA样本(病例组)和224份正常人样本(正常对照组),对MICA基因2~6外显子进行测序分型,并判读结果。分析MICA等位基因频率,跨膜区GCT重复次数,MICA-129Met/Val在正常对照组和病例组间的差异。结果发现19个MICA等位基因,与正常对照组比较,大多数MICA等位基因在各组间频率的差异无统计学意义。但MDS组的MICA*010:01频率明显低于正常对照组(P<0.01),而MDS组的MICA*019:01频率明显高于正常对照组、ALL组和AML组,差异均有统计学意义(P<0.01)。结论MICA*010:01和MICA*019:01的分布在MDS患者和正常人群间不同,提示这两个等位基因可能与MDS的易感性相关。

MICA基因多态性与乳腺癌细胞对NK细胞杀伤的敏感性

目的:探讨MHC-Ⅰ类链相关分子A(MHC class I chain-related molecule A,MICA)多态性与乳腺癌细胞对NK细胞杀伤敏感性的关系。方法:测序分析乳腺癌细胞系MCF-7、MDA-MB-231、MDA-MB-435S和SK-BR-3的MICA等位基因,用Western blotting和流式细胞术检测MICA重组表达载体转染293T细胞(分别命名为p MCFA5.1、p MCFA4、p231A5R、p231A9和p435A5P)MICA蛋白的表达水平,用LDH法检测NK细胞对转染MICA的293T细胞的杀伤活性,酶联免疫斑点法检测NK细胞穿孔素、颗粒酶B分泌水平。结果:MCF-7细胞表达MICA*008/A5.1和MICA*001/A4,MDA-MB-231和SK-BR-3细胞均表达MICA*019/A5和MICA*002/A9,MDA-MB-435S细胞表达MICA*010/A5。转染MICA后,p MCFA5.1组293T细胞MICA蛋白的表达水平最低(P<0.05),p435A5P组次之(P<0.05),p MCFA4组、p231A5R组和p231A9组表达水平较高(均P<0.05)。NK细胞对转染MICA的293T细胞杀伤活性及穿孔素、颗粒酶B分泌:p435A5P组对NK细胞杀伤的敏感性最低(P<0.05),穿孔素、颗粒酶B分泌水平最低(均P<0.05);p MCFA5.1、p MCFA4、p231A5R和p231A9各组之间比较差异无统计学意义(P>0.05)。结论:MICA基因多态性与乳腺癌细胞对NK细胞杀伤的敏感性密切相关。

MICA抗体与移植肾慢性失功的研究

目的 探讨肾移植术后患者抗主要组织相容性复合物I类相关链A基因（MICA）抗体与移植肾慢性失功的关系.方法 选择了1986年～2005年间在北京友谊医院接受肾移植的38例患者,男性32例,女性6例,年龄24～68岁,血肌酐和尿素氮水平高于正常值.采用MICA抗体流式筛查技术,于2009年7月检测MICA抗体和PRA抗体,38例肾移植患者PRA抗体均为阴性,而后观察一年后的肾功能变化.结果 38例肾移植术后群体反应性抗体阴性但血肌酐和尿素氮高于正常值的患者中有9例MICA抗体阳性,阳性率达23.68%.9例MICA抗体阳性患者均呈现MICA抗体多特异性.29例MICA抗体阴性患者,经过一年的治疗,7例患者肾功能基本恢复,2例患者恢复透析,20例患者肾功能基本未变.MICA抗体阳性的9例患者中有4例患者恢复透析,其MICA抗体均为强阳性;另5例患者肾功能基本未变,其MICA抗体4例为弱阳性,1例为阳性.MICA抗体阳性和MICA抗体阴性患者之间恢复透析的患者间差异有统计学意义（χ2=4.73,P〈0.025）.结论 高滴度MICA抗体是引起移植肾慢性失功的重要因素之一.

sMICA、CYFRA21-1、MMP9在食管鳞状细胞癌中的表达及与化疗疗效的关系

目的探讨可溶型主要组织相容性复合体Ⅰ类链相关蛋白A(sMICA)、细胞角质蛋白19片段抗原21-1(CYFRA21-1)、基质金属蛋白酶9(MMP9)在食管鳞状细胞癌中的表达情况及与化疗疗效的关系。方法选取经病理确诊的95例食管鳞状细胞癌患者的食管鳞状细胞癌组织,采用免疫组化SP连接法检测sMICA、CYFRA21-1、MMP9表达情况。化疗后评估疗效,分析sMICA、CYFRA21-1、MMP9的表达与化疗疗效的关系。结果95例食管鳞状细胞癌患者中,sMICA阳性表达59例(62.11%),CYFRA21-1阳性表达62例(65.26%),MMP9阳性表达75例(78.95%)。不同TNM分期、分化程度的食管鳞状细胞癌患者的食管鳞状细胞癌组织中sMICA、CYFRA21-1、MMP9阳性表达率比较,差异均有统计学意义(P﹤0.05)。95例患者化疗后,总有效率为58.95%,sMICA、CYFRA21-1、MMP9阴性表达的患者疗效优于阳性表达的患者,差异均有统计学意义(P﹤0.05)。多元Cox回归分析结果显示,TNM分期、分化程度、sMICA、CYFRA21-1、MMP9表达均是食管鳞状细胞癌患者化疗疗效的独立影响因素(P﹤0.01)。结论肿瘤标志性分子sMICA、CYFRA21-1、MMP9在食管鳞状细胞癌中阳性表达率高,与患者TNM分期、分化程度及化疗疗效密切相关。

白血病与尿毒症患者MICA*008基因分析

目的探讨MICA*008基因在白血病与尿毒症患者中的分布。方法应用PCR/SSP的方法检测白血病患者66例,尿毒症患者91例和无血缘关系健康人81例的MICA*008基因。结果白血病患者、尿毒症患者和正常健康人的MICA*008基因频率分别为22.2%,18.8%和34.3%。前两者的基因频率无差异(P>0.05),但均低于后者(P<0.05)。结论白血病和尿毒症患者的MICA*008基因频率均低于正常健康人,但两者之间无差异。

肾移植术后供受者MICA抗体对早期移植肾功能的影响

目的探讨供受者主要组织相容性复合物I类相关链A(MICA)抗体对肾移植术后早期移植肾功能的影响。方法采用Luminex200液相芯片技术,对43对肾移植供受者进行MICA抗体检测,其中26例尸体供者,所对应的43例受者。分为四组:(1)供受者均为MICA抗体阳性组;(2)供者MICA抗体阳性、受者MICA抗体阴性组;(3)供者MICA抗体阴性、受者MICA抗体阳性组;(4)供受者均为MICA抗体阴性组。比较各组之间术后急性排斥反应(AR)发生率、1周时血肌酐水平、移植肾功能恢复时间等资料,分析供受者MICA抗体对早期移植肾功能的影响。结果 26例尸体供者中MICA抗体阳性者5例(19.2%),抗体特异性频率最高的是MICA*019(40%);43例受者中MICA抗体阳性者11例(25.6%),抗体特异性频率最高的是MICA*018(14.6%)。43例受者肾移植后AR分析显示,第1组未发生AR(0/1);第2组AR发生率为33.3%(2/6),第3组AR发生率为40%(4/10);第4组AR发生率为38.4%(10/26)。各组之间AR发生率无统计学意义(P>0.05);各组在术后1周时血肌酐水平以及移植肾功能恢复时间方面无统计学意义(均P>0.05)。结论供受者任何一方在肾移植前存在MICA抗体对术后早期受者的AR发生率和肾功能恢复无明显影响。

高龄肾移植患者抗HLA抗体和MICA抗体对肾功能的影响

目的分析年龄大于60岁的肾移植患者术后PRA和MICA抗体对移植肾功能的影响。方法选择>60岁的高龄肾移植患者179例,对血清标本进行PRA和MICA抗体检测,并观察移植肾功能。结果 179例高龄肾移植患者中,抗体阳性患者32例(17.88%)。其中肾功能下降患者28例(87.5%)。抗体阴性患者147例中,肾功能下降患者7例(4.76%)。抗体阳性的肾移植患者,其移植肾功能下降率高于抗体阴性者,差异具有统计学意义(χ2=10.763,P<0.000 1)。移植肾存活大于10年以上的高龄患者91例,抗体阳性患者16例;移植肾存活未达10年以上的高龄患者88例,抗体阳性患者16例,两组患者抗体阳性率的差异无统计学意义(χ2=0.008 2,P>0.05)。移植肾存活已大于10年以上的患者中13例PRA抗体阳性,3例MICA抗体阳性,1例为抗HLA-Ⅰ+Ⅱ类和MICA阳性。16例抗体阳性患者移植肾功能均有不同程度下降。移植肾存活未达到10年的患者中15例PRA阳性,3例患者肾功能正常,为抗HLA-Ⅱ类阳性;12例患者移植肾功能均不同程度下降。结论抗HLA抗体和MICA抗体影响移植肾长期存活。肾移植术后动态监测抗HLA抗体和MICA抗体的变化,对预测移植肾排斥反应的发生、指导临床治疗、预防移植肾功能减退具有重要意义。

MICA抗体对移植肾功能的影响

目的研究肾移植术后患者抗主要组织相容性复合物I类相关链A(MICA)抗体与移植肾存活的关系。方法选择经检测证实群体反应性抗体(PRA)阴性的153例肾移植患者为该组研究对象。于2009年12月检测MICA抗体,而后观察3年后肾移植患者肾功能变化。结果 153例肾移植患者中,14例MICA抗体阳性,占9.2%;139例MICA抗体阴性,占90.8%。MICA抗体阳性患者肾功能异常率明显高于MICA抗体阴性患者(χ2=64.70,P<0.01)。结论 MICA抗体是引起移植肾慢性失功能的重要因素之一。

血管内皮细胞MICA基因的表达及其临床意义

目的 探讨内皮细胞MHC-I类链相关基因A（MICA）的表达及其临床意义.方法 对人脐静脉内皮细胞（HUVEC）和HeLa细胞进行培养,采用RT-PCR方法检测内皮细胞MICA mRNA表达、Western blot法检测MICA总蛋白和流式细胞仪检测MICA蛋白在细胞膜表叫的表达,用ELISA法测定细胞上清液中可溶性MICA（sMICA）的水平.结果 HUVEC和HeLa均有MICA mRNA和总蛋白的表达.HUVEC细胞表而的MICA分子表达（6.0%）明显低于HeLa细胞（37.0%）,差异有统计学意义（P〈0.05）.HUVEC细胞sMICA水平为352.5pg/mL,HeLa细胞为564.8pg/mL,两组之间差异有统计学意义（P〈0.05）.结论 内皮细胞MICA mRNA和总蛋向呈中度表达,但MICA膜蛋白表达较低.

IL-17A对肝细胞癌可溶性MICA表达的影响

目的:探讨患者外周血清白介素-17A(serum Interleukin-17A,IL-17A)对肝癌细胞可溶性MICA(soluble major histocompatibility complex class Ichain-related gene A,sMICA)的调控作用及可能机制.方法:收集慢性肝炎(chronic hepatitis,CH)、肝硬化(liver cirrhosis,LC)、HCC、健康对照者(healthcontrol,HC)各30例,采用ELISA方法分别检测血清sMICA及IL-17A的表达水平;HepG2和PLC/PRF/5细胞加入0、10、50ng/mL的重组人IL-17A(RhIL-17A)作用24h后,分别采用ELISA检测sMICA的表达;并在50ng/mL的RhIL-17A作用24h后,采用流式细胞术(flow cytometry,FCM)检测膜型MICA的表达、荧光定量RT-PCR检测MICA mRNA的表达、Western blot检测ADAM9,p65和磷酸化p65(P-p65)的表达.结果:HCC组血清IL-17A与sMICA水平明显高于CH、LC、HC组(IL-17AF=46.321,sMICAF=24.144,P<0.01),且二者呈正相关(r=0.28,P<0.01);RhIL-17A显著增加HCC细胞sMICA、膜MICA mRNA的表达(P<0.05),且可增加HCC细胞ADAM9和P-p65蛋白的表达.结论:IL-17A能上调肝癌细胞MICA mRNA表达,可能与其活化NF-B-ADAM9信号通路,从而增加HCC sMICA的表达有关.

结肠直肠癌患者围手术期NK细胞活化性受体NKG2D与其配体MICA/B的表达

目的观察结肠直肠癌(CRC)患者手术前后自然杀伤细胞(NK细胞)活化性受体NKG2D与其配体MICA/B的表达,探讨NKG2D-MIC系统与肿瘤逃避免疫监视的关系。方法流式细胞术检测45例CRC患者和35例健康体检者(对照组)外周血NK细胞活化性受体NKG2D的表达,组织MICA/B的表达;ELISA检测血清MICA(sMICA)的浓度。结果 CRC组术前NKG2D、MICA/B的表达均降低,sMICA浓度增高,与对照组比较差异均有统计学意义(P<0.05)。术后NKG2D的表达无显著增高,sMICA浓度无显著降低,与对照组比较差异均无统计学意义(P>0.05)。结论 CRC患者血清高水平的sMICA,抑制了NKG2D-MIC介导的抗肿瘤免疫,导致CRC患者NK细胞抗肿瘤免疫低下。NKG2D低表达,sMICA高浓度的情况术后短期内不能迅速逆转。