Relationship of human leukocyte antigen class II genes with the susceptibility to hepatitis B virus infection and the response to interferon in HBV-infected patients

AIM: To study the relationship of human leukocyte antigen (HLA)-DRB1 and -DQB1 alleles with the genetic susceptibility to HBV infection and the response to interferon (IFN) in HBV-infected patients.METHODS: Low-resolution DNA typing kit was used to determine HLA-DR-1 and -DQB1 genes in 72 patients with chronic hepatitis B (CHB) and HLA-DRB1 in 200 healthy people ready to donate their bone marrow in Shanghai.Among CHB patients, 35 were treated with IFNα-1b for 24 wk.RESULTS: The frequencies of HLA-DRB1*06, DRB1*08and DRB1*16 alleles in 72 patients were higher than in 200 healthy people (2.08% vs0%, OR = 3.837, P= 0.018;11.11% vs5.50%, OR = 2.148, P= 0.034; and 6.94% vs 3.00%, OR = 0.625, P = 0.049, respectively); whereas that of DRB1*07 allele was lower (2.78% vs 7.75%,OR = 0.340, P = 0.046). The frequency of HLA-DRB1* 14allele was higher in 11 responders to IFN compared with 24 non-responders (18.18% vs2.08%, OR = 10.444,P = 0.031), whereas that of DQB1*07 allele was inverse (9.09% vs 37.50%, OR = 0.167, P= 0.021).CONCLUSION: The polymorphism of HLA class Ⅱ may influence the susceptibility to HBV infection and the response to IFN in studied CHB patients. Compared with other HLA-DRB1 alleles, HLA-DRB1*06, DRB1*08, and DRB1*16 may be associated with chronicity of HBV infection, HLA-DRB1*07 with protection against HBV infection, and HLA-DRB1*14 allele may be associated with a high rate of the response of CHB patients to IFN treatment.Compared with other HLA-DQB1 alleles, HLA-DQB1*07 may be associated with low response rate to IFN.

Impact of human leukocyte antigen matching on hepatitis B virus recurrence after liver transplantation

BACKGROUND: Liver transplantation (LT) is an effective therapy for end-stage hepatitis B virus (HBV) infection. Recurrence of HBV is one of the frequent complications. In the present study, we investigated whether human leukocyte antigen (HLA) matching influences the incidence of HBV recurrence, and the time point of HBV recurrence after LT. METHODS: One hundred and two recipients of LT with end-stage chronic HBV infection were reviewed. The triple-drug immunosuppression regimen consisted of tacrolimus, mycophenolate, and prednisone. All patients were subjected to prophylaxis with hepatitis B immunoglobulin and lamivudine. HLA typing was performed using a sequence-specific primer-polymerase chain reaction kit. Serology for hepatitis B and HBV DNA was examined using a commercial kit. RESULTS: The incidence of recurrent HBV infection post-LT was 6.86%. The recurrent infection of HBV was independent of the degree of H LA matching (P>0.05). The time point of HBV recurrence, however, was prolonged in HLA-A matched patients compared with matchless patients (P=0.049). The recurrence of HBV infection was independent of H LA compatibility. CONCLUSIONS: This retrospective analysis showed that more HLA-A locus compatibility is associated with a prolonged time of recurrence of HBV in patients after LT for end-stage HBV infection. The incidence of HBV recurrence is independent of HLA compatibility. (Hepatobiliary Pancreat Dis Int 2010; 9: 139-143)

Association of human leukocyte antigen DQB1 and DRB1 alleles with chronic hepatitis B

AIM: To investigate the effect of human leukocyte antigen(HLA) DRB1 and DQB1 alleles on the inactive and advanced stages of chronic hepatitis B.METHODS: Patient records at a single institution's hepatology clinic were reviewed. Demographic data, laboratory results, endoscopy results, virological parameters, biopsy scores and treatment statuses were recorded. In total, 355 patients were eligible for thestudy, of whom 226(63.7%) were male. Overall, 82(23.1%) were hepatitis B early antigen(HBeAg) positive, 87(24.5%) had cirrhosis, and 66(18.6%) had inactive disease. The presence of DQB1 and DRB1 alleles was determined by polymerase chain reaction with sequence-specific primers. The distribution of the genotyped alleles among patients with cirrhosis and patients with chronic active hepatitis was analyzed.RESULTS: The most frequent HLA DQB1 allele was DQB1*03:01(48.2%), and the most frequent HLA DRB1 allele was DRB1*13/14(51.8%). DQB1*05:01 was more frequent in patients with active disease than in inactive patients(27% vs 9.1%; P = 0.002, Pc = 0.026). DRB1*07 was rare in patients with cirrhosis compared with non-cirrhotics(3.4% vs 16%; P = 0.002, Pc = 0.022). Older age(P < 0.001) and male gender(P = 0.008) were the other factors that affected the presence of cirrhosis. In a multivariate logistic regression analysis, DRB1*07 remained a significant negative predictor of cirrhosis(P = 0.015). A bioinformatics analysis revealed that a polymorphic amino acid sequence in DRB1*07 may alter interaction with the T-cell recognition site.CONCLUSION: This study demonstrates that HLA alleles may influence cirrhosis development and disease activity in Turkish chronic hepatitis B patients.

Occurrence of human leukocyte antigen B51-related ankylosing spondylitis in a family:Two case reports

BACKGROUND Ankylosing spondylitis(AS)is strongly associated with the human leukocyte antigen(HLA)B27 haplotype.In regions where conventional polymerase chain reaction for HLA typing is available for antigens such as HLA B27 or HLA B51,it is common to perform the HLA B27 test for evaluation of AS.While HLA B27-associated clustered occurrences of AS have been reported in families,we report the first case series of HLA B51-related occurrences of AS in a family.CASE SUMMARY A father and his daughters were diagnosed with AS and did not have the HLA B27 haplotype.Although they were positive for HLA B51,they exhibited no signs of Behçet’s disease(BD).Of the five daughters,one had AS,and three,including the daughter with AS,were positive for HLA B51.The two daughters with the HLA B51 haplotype(excluding the daughter with AS)exhibited bilateral grade 1 sacroiliitis,whereas the daughters without the HLA B51 haplotype did not have sacroiliitis.Thus,this Korean family exhibited a strong association with the HLA B51 haplotype and clinical sacroiliitis,irrespective of the symptoms of BD.CONCLUSION It is advisable to check for HLA B51 positivity in patients with AS/spondyloarthropathy who test negative for HLA B27.

Human leukocyte antigen-DP loci are associated with the persistent infection of hepatitis B virus in Chinese population

A genome-wide association study recently showed that genetic variants in human leukocyte antigen (HLA)-DP loci were strongly associated with a risk of persistent infection of hepatitis B virus (HBV) in Japanese and Thai individuals and variants in interleukin 28B (IL-28B) have been associated with responses to anti-hepatitis C virus (HCV) treatment. The aim of this study was to investigate whether the HLA-DP loci and IL-28B were associated with different outcomes of chronic HBV infection (CHB) in Chinese subjects. The rs9277535 near HLA-DPB1,rs3077 near HLA-DPA1, and rs12979860 near IL-28B were genotyped by direct sequencing in 185 CHB patients and 193 self-limited hepatitis B virus (SLHBV)-infected subjects who recovered from HBV infection. The rs9277535 near HLA-DPB1 was strongly associated with CHB (P=0.000 018 1, OR=1.905). This association was observed independent of HBV e antigen (HBeAg) status and HBV viral loads in HBeAg-positive CHB patients (P=0.000 4, OR=1.956), in HBeAg-negative CHB patients (P=0.000 9, OR=1.857), and in HBeAg-negative CHB individuals without detectable levels of HBV DNA in serum (P=0.001 1, OR=2.05). The rs3077 near HLA-DPA1 was associated with CHB (P=0.020 6, OR=0.686 5) and HBeAg-positive CHB infection status (P=0.014 3, OR=0.604 7). Meanwhile, a genetic variation of insertion-deletion (INDEL) polymorphism (rs361527, -/ATAAATGTTGA) near HLA-DPA1 was found to be associated with CHB (P=0.030 7, OR=0.702 8) and HBeAg-positive CHB infection status (P=0.023 3, OR=0.619). However,the rs12979860 genotype near IL-28B had no correlation with CHB. This study demonstrated that in the Han Chinese populations, HLA-DP loci, but not IL-28B, were associated with persistence of infection in different outcomes of HBV-infected patients; however, the mechanism needs to be further investigated.

Reflections on the prevalence of human leukocyte antigen-B27 and human leukocyte antigen-B51 co-occurrence in patients with spondylarthritis

We performed a literature mini-review of the clinical profile of patients with spondylarthritis who are also human leukocyte antigen(HLA)-B51-positive.It seems to us that patients with HLA-B27 and HLA-B51 are more common in men,Asians and between the third and ninth decades of life.They are more likely to develop peripheral joint conditions,with cutaneous manifestations(e.g.,oral ulcers)and uveitis.Therefore,more robust epidemiological studies with more accurate methodology and multicenter locations are needed to better map the role of the interaction between HLA-B51 in patients with spondylarthritis.

HLA-B和-DRB1、HLA-DQB1和-DPB1座位基因重组的分析

目的:探讨2个家系人类白细胞抗原(HLA)座位的重组情况。方法:采集家系成员的外周血,提取基因组DNA,采用聚合酶链反应-序列特异性寡核苷酸探针技术(PCR-SSO)和二代测序技术检测HLA-A、-B、-C、-DRB1、-DQB1和-DPB1座位,通过家系遗传分析确定个体HLA单体型。结果:家系1中单体型HLA-A*11:01~C*03:04~B*13:01~DRB1*12:02~DQB1*03:01~DPB1*05:01:01G与HLA-A*03:01~C*04:01~B*35:03~DRB1*12:01~DQB1*03:01~DPB1*04:01:01G在HLA-B和HLA-DRB1座位间进行了交换,形成HLA-A*11:01~C*03:04~B*13:01~DRB1*12:01~DQB1*03:01~DPB1*04:01:01G。家系2中单体型HLA-A*02:06~C*03:03~B*35:01~DRB1*08:02~DQB1*04:02~DPB1*13:01:01G与HLA-A*11:01~C*07:02~B*38:02~DRB1*15:02~DQB1*05:01~DPB1*05:01:01G在HLA-DQB1和HLA-DPB1座位间进行了交换,形成HLA-A*02:06~C*03:03~B*35:01~DRB1*08:02~DQB1*04:02~DPB1*05:01:01G。结论:2个中国汉族人群家系分别发生了HLA-B和-DRB1、HLA-DQB1和-DPB1座位间的基因重组。

HLA-B基因rs1058026和rs3819299位点单核苷酸多态性与女性强直性脊柱炎易感性的关系

目的探讨人类白细胞抗原(HLA)-B基因rs1058026和rs3819299位点单核苷酸多态性与女性强直性脊柱炎(AS)易感性的相关性。方法选取108例女性AS患者(病例组)及129例体检正常女性(对照组)。比较两组研究对象的一般资料,以及HLA-B基因rs1058026和rs3819299位点基因型和等位基因分布频率。使用Logistic回归模型分析上述基因位点基因型和等位基因与女性AS易感性的相关性。结果病例组AS家族史比例及HLA-B27阳性比例均高于对照组(均P<0.05),而两组吸烟史比例、饮酒史比例差异均无统计学意义(均P>0.05)。HLA-B基因rs3819299位点的等位基因G增加女性的AS发病风险(OR=16.172,P<0.05),相比于基因型TT,rs3819299位点的基因型GT增加女性的AS发病风险(OR=113.877,P<0.05);HLA-B基因rs1058026位点的等位基因和基因型与女性的AS发病风险无关(均P>0.05)。结论HLA-B基因rs3819299位点单核苷酸多态性与女性AS易感性相关,rs3819299位点的等位基因G、基因型GT可能会增加女性AS的发病风险。

湖南地区携带HLA-B*27꞉04等位基因人群与强直性脊柱炎的易感性具有强相关性

目的:人类白细胞抗原(human leukocyte antigen,HLA)B27是强直性脊柱炎(ankylosing spondylitis,AS)的易感等位基因,HLA-B27抗原分型是临床诊断AS的重要指标,但目前的分型方法如序列特异引物聚合酶链反应技术(polymerase chain reaction-sequence specific primer,PCR-SSP)等仍存在一定的缺陷。因此,本研究旨在应用高分辨率聚合酶链反应直接测序分型法(polymerase chain reaction-sequence-based typing,PCR-SBT)分析B27亚型与湖南地区强直性脊柱炎易感性的相关性。方法:收集2020年1至12月在湘雅二医院门诊就医的116例疑似AS患者(疑似AS组)和121名健康志愿者(对照组)的外周血,采用PCR-SBT进行HLA-B基因分型。在疑似AS组患者中,23名患者最终被确诊为AS(AS确诊组),其余的93名未能确诊的患者为非AS确诊组。采用PCR-SBT和PCR-SSP检测116例疑似AS患者的HLA-B27分型,并比较2种方法的检测结果。结果:疑似AS组HLA-B27等位基因频率显著高于对照组[11.63%vs 2.48%;P<0.001,优势比(odds ratio,OR)=5.18,95%置信区间(confidence interval,CI)2.097~12.795]。疑似AS组和对照组均检出B*27:04、B*27:05、B*27:06、B*27:07。疑似AS组B*27:04等位基因频率明显高于对照组[9.48%vs 1.24%;P<0.001,OR=8.346,95%CI 2.463~28.282]。疑似AS组和AS确诊组B27阳性率(B27+/+和B27+/-)均显著高于对照组(分别χ^(2)=16.579,P<0.001;χ^(2)=94.582,P<0.001)。在AS确诊组中,21例为HLA-B27携带者,AS确诊组B27阳性率为91.3%。PCR-SBT方法可对HLA-B基因位点进行高分辨分型,其敏感度、特异度、阳性预测值、阴性预测值、准确度均高于PCR-SSP法。结论:应用PCR-SBT检测出HLA-B*27:04与湖南地区AS具有强相关性。PCR-SBT可作为临床AS辅助诊断的优选方案。

长链非编码RNA人类白细胞抗原复合体18通过微RNA-497-5p/细胞周期蛋白E1轴调节弥漫性大B细胞淋巴瘤的增殖、凋亡和侵袭

目的 探讨长链非编码RNA人类白细胞抗原复合体18(lncRNA HCG18)调控微RNA-497-5p(miR-497-5p)/细胞周期蛋白E1(CCNE1)轴对弥漫性大B细胞淋巴瘤(DLBCL)细胞增殖、凋亡和侵袭的影响。方法 实时荧光定量PCR(qRT-PCR)、蛋白质印迹法分别检测2018年5月至2021年5月收集的恩施土家族苗族自治州中心医院DLBCL病人淋巴组织、良性淋巴结增生病人的淋巴组织、人正常B细胞永生化细胞HMy2.CIR、DLBCL细胞系SU-DHL-1、OCI-LY8、U2932中HCG18、miR-497-5p表达及CCNE1蛋白表达,将OCI-LY8细胞分为Ct组(正常培养的OCI-LY8细胞)、pcDNA组(细胞转染过表达物阴性对照)、pcDNA-HCG18组(细胞转染HCG18过表达物)、si-NC组(细胞转染小干扰RNA阴性对照)、si-HCG18组(细胞转染HCG18小干扰RNA)、si-HCG18+inhibitorNC组(细胞转染HCG18小干扰RNA和抑制物阴性对照)、si-HCG18+miR-497-5p inhibitor组(细胞转染HCG18小干扰RNA和miR-497-5p抑制物),CCK-8法检测细胞增殖,流式细胞术检测细胞凋亡,Transwell检测细胞侵袭,蛋白质印迹法检测CCNE1、增殖细胞核抗原(PCNA)、Bcl-2相关X蛋白(Bax)、基质金属蛋白酶9(MMP-9)蛋白表达,双萤光素酶验证HCG18与miR-497-5p、miR-497-5p与CCNE1的关系。结果 在DLBCL淋巴组织和细胞中,HCG18、CCNE1蛋白高表达,miR-497-5p低表达,且在OCI-LY8细胞中HCG18、CCNE1蛋白表达上调最高,miR-497-5p表达下调最多(P<0.05),因此,以OCI-LY8细胞进行后续研究,与si-NC组比较,si-HCG18组HCG18(0.26±0.03比1.01±0.01)、CCNE1蛋白(0.45±0.03比1.44±0.19)表达降低,miR-497-5p(1.95±0.14比1.03±0.02)表达升高(P<0.05),与pcDNA组比较,pcDNA-HCG18组HCG18(1.96±0.23比1.02±0.01)、CCNE1蛋白(2.33±0.21比1.42±0.18)表达升高,miR-497-5p(0.28±0.02比1.02±0.02)表达降低(P<0.05),与siHCG18组、si-HCG18+inhibitor NC组比较,miR-497-5p表达降低(1.21±0.09比1.95±0.14、1.94±0.13),CCNE1蛋白(0.87±0.08比0.45±0.03、0.44±0.04)表达上调(P<0.05),沉默HCG18可抑制OCI-LY8细胞增殖、侵袭行为及PCNA、MMP-9蛋白表达,诱导细胞凋亡及Bax蛋白表达,而上调HCG18则呈相反趋势,下调miR-497-5p逆转了沉默HCG18对OCI-LY8细胞增殖、侵袭、凋亡的影响,HCG18靶向调控miR-497-5p/CCNE1。结论 沉默HCG18可能通过调控miR-497-5p/CCNE1抑制OCI-LY8细胞增殖、侵袭,诱导细胞凋亡。

HLA-B对喉癌Hep2细胞生物学行为的影响

目的探讨人类白细胞组织相容抗原(HLA)-B在喉癌发生、发展中的作用。方法采用RNA干涉技术下调Hep2细胞中HLA-B基因表达。用干涉效应最明显、转染siRNA的细胞作为观察组,转染PBS及无义siRNA的细胞作为对照1组及对照2组。采用流式细胞仪、MTT和细胞体外侵袭力分析方法检测各组细胞凋亡率、增殖情况、细胞周期及局部侵袭能力。结果 RNA干涉7 d观察组细胞凋亡率明显高于两对照组,细胞周期阻滞于S期;细胞增殖能力及局部侵袭能力明显强于两对照组,P均<0.05。结论 HLA-B表达降低或缺失在喉癌的发生、发展中起促进作用。

人类白细胞抗原基因HLA-B*58∶01基因型的快速低成本鉴别方法

采用焦磷酸测序技术和改进的全血基因组提取方法,建立了位于6号染色体的银屑病易感基因1候选基因1(Psoriasis susceptibility 1 candidate 1,PSORS1C1)rs9263726位点的焦磷酸测序方法,检出限达到0.4 ng/μL基因组DNA,20例标本的焦磷酸法和Sanger法测序结果完全一致。利用本方法对683例标本的rs9263726位点进行测序,得到中国人群该位点野生型(GG型)分布频率为87.6%,突变的GA型分布频率为11.7%、AA型分布频率为0.7%。通过对随机选取的46例标本rs9263726位点与人类白细胞抗原基因HLA-B*58∶01基因型的连锁关系进行分析,结果表明,该位点预测HLA-B*58∶01基因型的灵敏度为100%、特异性为91.3%。本方法可用于HLA-B*58∶01基因型的检测。

HLA新等位基因HLA-B* 13∶42的确认及序列分析

目的认定1个人类白细胞抗原(HLA)新等位基因并分析其核苷酸序列。方法应用PCR-SBT进行HLA常规分型发现1个与HLA-B*13相关的异常等位基因,用针对于B*13的位点特异性SSSP引物测序,确认与同源性最高的HLA等位基因序列的差异。结果发现1个标本的HLA-B位点核苷酸序列与所有已知HLA-B位点等位基因核苷酸序列不一致,与同源性最高的等位基因B*13:02:01的差异是在第3外显子445位的G>T,其突变导致密码子GCC>TCC,结果造成B*13:02:01氨基酸序列中125位的Ala丙氨酸(A)变为丝氨酸(S)。结论该等位基因为HLA-B位点的1个新等位基因,该基因被世界卫生组织(WHO)HLA命名委员会命名为HLA-B*13:42。

外周血单个核细胞表面HLA-A和HLA-B在结直肠肿瘤中的表达

目的检测外周血单个核细胞表面(PBMC)HLA-A和HLA-B在结直肠肿瘤患者中的表达,并探讨其在肿瘤发生发展中的作用。方法以Beta-actin为内参照,实时荧光定量RT-PCR方法检测结直肠肿瘤患者(结直肠肿瘤组,n=50)、结直肠良性病变患者(良性病变组,n=35)和健康体检者(正常对照组,n=42)外周血单个核细胞HLA-A和HLA-B mRNA的表达,并比较结直肠肿瘤不同TNM分期中HLA-A和HLA-B mRNA的表达。三组平均年龄相近。用Rest(relative expression software tool)软件计算相对表达率(Ratio)。结果正常对照组PBMC的HLA-A和HLA-B mRNA相对表达率分别为0.99±0.47,1.13±0.60;结直肠良性病变组相对表达率分别为0.76±0.59,0.84±0.57;结直肠肿瘤组分别为0.38±0.31和0.39±0.35。结直肠肿瘤组PBMC的HLA-A mRNA和HLA-B mR-NA相对表达率低于正常对照组和结直肠良性病变组(P<0.001)。结直肠肿瘤组HLA-A mRNA在TNM不同分期之间的表达无统计学差异(P>0.05);HLA-B mRNA在TNMⅠ期患者中的表达高于Ⅱ期和Ⅳ期(P<0.05),在其他不同分期之间差异无统计学意义(P>0.05)。结论结直肠肿瘤患者外周血单个核细胞HLA-A和HLA-B与其细胞免疫相关,在抗肿瘤免疫中起重要作用。

HLA新等位基因HLA-B*35:155的确认

目的发现和认定一个人类白细胞抗原(HLA)新等位基因。方法应用多聚酶链式反应—基于测序的分型技术(polymerase chain reaction-sequence based typing,PCR-SBT)进行HLA常规分型,HLA-B位点分型结果与等位基因B*35:03:01,51:01:01在112位有一个碱基不匹配,不能指定为任何HLA-B位点等位基因,用针对于B*35、B*51的序列特异性SSSP引物测序,确认与同源性最高的HLA等位基因序列的差异。结果测序结果表明该等位基因与其同源性最高的等位基因B*35:03:01的差异是在第2外显子112位的C>T,其突变导致密码子CGG>TGG,结果造成B*35:03:01氨基酸序列中14位的精氨酸(R)变为色氨酸(W)。结论该等位基因为HLA-B位点的一个新等位基因,世界卫生组织(WHO)HLA命名委员会将其正式命名为HLA-B*35:155。

HLA-B在口腔鳞状细胞癌中的表达及意义

目的通过检测人类白细胞抗原B(human leukocyte antigen B,HLA-B)在口腔鳞状细胞癌(oral squamous cell carcinoma,OSCC)原发灶、转移灶以及口腔正常黏膜、癌前病变中的表达情况,探讨其在口腔鳞癌发生、发展和淋巴道转移中的作用。方法应用免疫组织化学方法检测70例OSCC组织、14例癌前病变组织以及10例正常组织的HLA-B表达,比较OSCC的不同病理分级、TNM分期、有无淋巴结转移、原发灶和转移灶、正常及癌前病变组织HLA-B的表达情况。结果 HLA-B在正常组织、癌前病变组织、癌组织的表达逐渐下降(P<0.05);其中,癌分化等级越低,HLA-B表达量越低;正常组织、癌前病变组织和高分化OSCC之间的表达无明显差异,但明显高于中、低分化OSCC(P<0.05);不同T分期之间差异无统计学意义(P>0.05);原发灶与转移灶HLA-B表达差异亦无统计学意义(P>0.05)。但是,未出现转移的OSCC原发灶HLA-B表达高于出现转移的原发灶(P=0.069)。结论中、低分化OSCC组织HLA-B表达较正常组织、癌前病变以及高分化OSCC明显下调,与中、低分化OSCC较高的淋巴道转移率相关,提示HLA-B的表达减弱可能通过肿瘤免疫逃逸机制在OSCC淋巴道转移中有着重要意义,HLA-B表达可作为一项监测OSCC恶性程度与淋巴道转移的指标。

PBMC中PD-L1、HLA-B、MRP5在晚期乳腺癌放疗过程中的动态表达及意义

目的探究外周血单个核细胞(PBMC)中程序性细胞死亡配体1(PD-L1)、人类白细胞抗原-B(HLA-B)、多药耐药相关蛋白5(MRP5)在晚期乳腺癌放疗过程中的动态表达及意义。方法选取保山市人民医院122例晚期乳腺癌患者,根据放疗结束后4周评估疗效,分为有效组(74例)与无效组(48例),放疗过程中动态监测PBMC中PD-L1、HLA-B、MRP5 mRNA水平,分析其临床意义。结果放疗1个疗程、放疗结束后PBMC中PD-L1、MRP5 mRNA水平低于放疗前,HLA-B mRNA水平高于放疗前(P<0.05);有效组放疗1个疗程、放疗结束后PBMC中PD-L1、MRP5 mRNA水平低于无效组,HLA-B mRNA水平高于无效组,放疗前与放疗结束后PBMC中PD-L1、MRP5、HLA-B mRNA水平差值绝对值高于无效组(P<0.05);PBMC中PD-L1、HLA-B、MRP5 mRNA水平放疗前与放疗结束后差值绝对值呈正相关(P<0.05);放疗前与放疗结束后PBMC中PD-L1、MRP5、HLA-B mRNA水平差值绝对值与疗效呈正相关(P<0.05);PBMC中PD-L1、HLA-B、MRP5 m RNA差值绝对值联合预测疗效的AUC为0.951,95%CI为0.906~0.996,敏感度为91.67%,特异度为91.89%,优于各指标单独预测(P<0.05)。结论晚期乳腺癌放疗过程中动态监测PBMC中PD-L1、MRP5、HLA-B mRNA水平变化情况能作为临床预测疗效的潜在途径,有助于及时调整放疗方案、提高疗效。

Association of human leukocyte antigen-DR-DQ-DP haplotypes with the risk of hepatitis B virus-related hepatocellular carcinoma

Aim:Genetic polymorphisms of human leukocyte antigen(HLA)class II molecules are associated with chronic hepatitis B virus(HBV)infection.We aimed to investigate the impacts of HLA-II haplotypes on viral evolution and the risks of HBV-caused liver diseases.Methods:HLA-DR-DQ-DP haplotypes were estimated in 1210 healthy controls,296 HBV clearance subjects,301 asymptomatic hepatitis B surface antigen carriers,770 chronic hepatitis B patients,443 HBV-related liver cirrhosis(LC)patients,and 1037 HBV-related hepatocellular carcinoma(HCC)patients.HBV mutations were determined by sequencing.The associations of HLA-DR-DQ-DP haplotypes with viral mutations and the risks of liver diseases were assessed by multivariate logistic regression.Results:Compared to HBV-free subjects,the haplotypes CCAACG,CCGACG,TCAATA,and TCGATA were associated with decreased HCC risk,with an odds ratio(OR)[95%confidence interval(CI)]of 0.62(0.40-0.95),0.60(0.39-0.92),0.73(0.54-0.98),and 0.58(0.42-0.78),respectively.CCAACG,CCGACG,and TCAATA were significantly associated with decreased frequencies of the HCC-risk HBV mutations:preS1 deletion,APOBECsignature HBV mutations in the core promoter and preS regions,A51C/T,G104C/T,and G146C/T.TCGATA and TTAACG were associated with increased LC risk,with an OR(95%CI)of 1.54(1.03-2.30)and 2.23(1.50-3.33),respectively.However,TCGATA and TTAACG were not consistently associated with the cirrhosis-risk HBV mutations.Conclusion:CCAACG,CCGACG,and TCAATA are inversely associated with HCC risk,possibly because they are involved in creating an immune microenvironment attenuating the generation of HCC-risk HBV mutations.TCGATA and TTAACG might predispose the polarity of immunity towards Th17 isotype related to LC.

中医体质和HBV感染结局的关联及其与人类白细胞抗原-DQA1基因多态性的关系

目的观察中医体质类型与浙江地区汉族人群乙型肝炎病毒(HBV)感染不同临床状态及人类白细胞抗原(HLA)DQA1基因多态性的关系,探讨中医体质因素在慢性乙型肝炎发病中的作用。方法临床收集慢性乙型肝炎(CHB,120例)、慢性HBV携带者(ASC,60例)、自限性HBV感染者(RHBS,60例)3组患者,前两组诊断均经肝活检证实。以王琦体质分类判定中医体质类型;聚合酶链反应序列特异性引物(PCR-SSP)法检测HLA-DQA1基因型,比较组间体质类型分布的差异及组间基因频率的差异。结果(1)CHB组阴虚质、痰湿质的分布频率(20.0%、12.5%)显著高于RHBS组(6.7%、1.7%),平和质的分布频率(11.7%)显著低于RHBS组(31.7%),差异均有统计学意义(OR=3.500,95%CI:1.16-10.60;OR=8.400,95%CI:1.09-65.42;OR=0.161,95%CI:0.076-0.34;均P<0.05);(2)CHB组湿热质的分布频率(24.2%)显著高于ASC组(6.7%,P<0.05,OR=4.462,95%CI:1.49-13.36),平和质的分布频率(11.7%)显著低于ASC组(45.0%,P<0.01,OR=0.285,95%CI:0.13-0.62);(3)HLA-DQA1*0201在CHB组的分布频率(38.3%)显著高于RHBS组(5.8%,P<0.01,OR=10.04,95%CI:4.48-22.48);HLA-DQA1*0102的分布频率(9.6%)显著低于RHBS组(36.7%,P<0.01,OR=0.183,95%CI:0.10-0.32);(4)HLA-DQA1*0201在CHB组的分布频率(38.3%)显著高于ASC组(7.5%,P<0.01,OR=7.667,95%CI:3.7-15.87);HLA-DQA1*0102的分布频率(20%)显著低于ASC组(9.6%,P<0.01,OR=0.424,95%CI:0.23-0.79)。结论中医体质因素和HLA-DQA1基因多态性均可影响HBV感染的临床结局,但其间关系需进一步研究明确。

HBV感染者人类白细胞Ⅰ,Ⅱ类抗原等位基因多态性分析

目的:分析HBV感染者体内病毒持续和清除与HLA-A,B,DRB1各位点等位基因分布频率的关系.方法:采用序列特异性引物-聚合酶链式反应(PCR-SSP)技术,对61例慢性乙型肝炎患者(CHB)、32例HBV感染后病毒清除者(感染恢复组)和40例骨髓移植供者(正常组)的外周血白细胞,进行人类白细胞抗原等位基因(HLA-A,B,DRB1)分型检测.结果:在慢性乙型肝炎组,HLA-DRB1*12等位基因分布频率较正常组(0.230vs0.075,P=0.004,OR=3.674,95%CI:1.445-9.338)和HBV感染恢复组(0.230vs0.063,P=0.004,OR=4.468,95%CI:1.492-13.377)均显著增高,HLA-B*35,DRB1*13则显著降低(0.066vs0.163,P=0.027,OR=0.362,95%CI:0.143-0.918;0.016vs0.008,P=0.017,OR=0.174,95%CI:0.035-0.859);HLA-A*69,B*56也显著降低(均0.000vs0.037,P=0.031).HLA-A*02等位基因分布频率在慢性肝炎组与HBV感染恢复组比较显著降低(P=0.044),HLA-B*51在感染恢复组与正常组比较显著增高(P=0.019).结论:机体对HBV易感性和病毒持续或清除与HLA等位基因多态性相关.HLA-DRB1*12可能既为易感性位点,又能促进病毒的持续感染;HLA-B*51,A*02可能为易感性位点,但感染后易清除病毒;HLA-DRB1*13可能是抗HBV感染的保护性基因;HLA-B*35,B*56和A*69在中国北方汉族人可能也为抗HBV感染的保护性基因.