Clonal immunoglobulin heavy chain and T-cell receptor γ gene rearrangements in primary gastric lymphoma

AIM:To study the diagnostic value of immunoglobulin heavy chain(IgH)and T-cell receptorγ (TCR-γ)gene monoclonal rearrangements in primary gastric lymphoma(PGL).METHODS:A total of 48 patients with suspected PGL at our hospital were prospectively enrolled in this study from January 2009 to December 2011.The patients were divided into three groups(a PGL group,a gastric linitis plastica group,and a benign gastric ulcer group)based on the pathological results(gastric mucosal specimens obtained by endoscopy or surgery)and follow-up.Endoscopic ultrasonography(EUS)and EUSguided biopsy were performed in all the patients.The tissue specimens were used for histopathological examination and for IgH and TCR-γ gene rearrangement polymerase chain reaction analyses.RESULTS:EUS and EUS-guided biopsy were successfully performed in all 48 patients.In the PGL group(n=21),monoclonal IgH gene rearrangements were detected in 14(66.7%)patients.A positive result for each set of primers was found in 12(57.1%),8(38.1%),and 4(19.0%)cases using FR1/JH,FR2/JH,and FR3/JH primers,respectively.Overall,12(75%)patients with mucosal-associated lymphoid tissue lymphoma(n=16)and 2(40%)patients with diffuse large B-cell lymphoma(n=5)were positive for monoclonal IgH gene rearrangements.No patients in the gastric linitis plastica group(n=17)and only one(10%)patient in the benign gastric ulcer group(n=10)were positive for a monoclonal IgH gene rearrangement.No TCRgene monoclonal rearrangements were detected.The sensitivity of monoclonal IgH gene rearrangements was 66.7%for a PGL diagnosis,and the specificity was96.4%.In the PGL group,8(100%)patients with stage IIE PGL(n=8)and 6(46.1%)patients with stage IE PGL(n=13)were positive for monoclonal IgH gene rearrangements.CONCLUSION:IgH gene rearrangements may be associated with PGL staging and may be useful for the diagnosis of PGL and for differentiating between PGL and gastric linitis plastica.

Profiling the repertoire of T-cell receptor beta-chain variable genes in peripheral blood lymphocytes from subjects who have recovered from acute hepatitis B virus infection

The profile of T-cell receptor beta-chain variable （TRBV） genes usually skews in subjects with virus infection or cancer. The gene melting spectral pattern （GMSP） can be used to determine the profile of the TRBV gene family. To explore the portrait of the TRBV family in peripheral blood lymphocytes from subjects who have recovered from acute hepatitis B virus infection （AHI）, peripheral blood mononuclear cells （PBMCs） were separated and further sorted into CD4^＋ and CD8^＋ T-cell subsets. The molecular features of the TRBV complementary determining region 3 （CDR3） motifs were determined using GMSP analysis. When a GMSP profile showed a single peak, the monoclonally expanded TRBV gene was cloned and sequenced. Skewed expansions of multiple TRBV genes were observed among the CD4^＋ and CD8^＋ T-cell subsets and the PBMCs. The frequency of monoclonally expanded TRBV genes in the CD8^＋ T-cell subset was significantly higher than that of the CD4^＋ T-cell subset and the PBMCs. Compared to other members of the TRBV gene family, TRBV11, BV15 and BV20 were predominantly expressed in the repertoire of peripheral blood lymphocytes in recovered AHI subjects. The relatively conserved amino acid motifs of TRBV5.1 and BV20 CDR3 were also detected in the CD4^＋ and CD8^＋ T-cell subsets. These results demonstrate the presence of multiple biased TRBV families in recovered AHI subjects. TRBV11, BV15 and BV20, especially from the CD8＋ T-cell subset, may be relevant to the pathogenesis of subjects with AHh The preferentially selected TRBV5.1 and BV20 with the relatively conserved CDR3 motif may be potential targets for personalized treatments of chronic HBV infection.

Study on Cellular Differentiation and Genes Rearrangement of Malignant Lymphoproliferative Disorders

Malignant lymphoproliferative disorders are common diseases characterized by the clonal proliferation of cells derived from the lymphocytes of different developmental stages. The analyses of routine morphology and cytochemistry fail to determine the origin and differentiation stages. The cell differentiation origin of most of malignant lymphoproliferative disorders can be defined by using monoclonal antibodies(McAbs) against the differentiation antigens of lymphocytes, but it is unable to determine the cell origin of a minority of undifferentiated malignancies and also fails to distinguish the malig-

肝脾T细胞淋巴瘤临床病理学分析

目的:探讨肝脾T细胞淋巴瘤(hepatosplenic T cell lymphoma,HSTCL)的临床病理特征和病理诊断。方法:复习3例HSTCL患者的临床病理资料,免疫表型,EB病毒(Epstein-Barr virus,EBV)原位杂交及T细胞受体γ(T cell receptor γ,TCRγ)基因重排检测。结果:3例HSTCL中,骨髓1例呈间质和窦性浸润,2例呈间质及弥漫性浸润;肝1例和脾1例呈窦性浸润。免疫组化:3例均CD3、TIA-1强阳性,而粒酶B阴性;CD56阴性;TCRβ阴性;3例EBV原位杂交均阴性。TCRγ基因重排检测2例呈单克隆性,1例呈弥散态。结论:HSTCL是一种罕见的非活化T细胞毒性的外周T细胞淋巴瘤(peripheral T cell lymphoma,PTCL),EBV原位杂交阴性和TCRγ基因克隆性重排有助于诊断和鉴别诊断。我国病例与国际报道病例临床病理特征基本一致。

24例儿童非霍奇金淋巴瘤IgH和TCR基因重排的研究

目的检测２４例儿童非霍奇金淋巴瘤（ＮＨＬ）ＩｇＨ和ＴＣＲ基因重排，以便选择恰当的引物组合用于ＮＨＬＶＩ期患儿微小残留病（ＭＲＤ）的检测。方法以Ｃｈｅｌｅｘ１００为介质，从初诊的ＮＨＬ患儿病理切片中提取ＤＮＡ，采用聚合酶链反应（ＰＣＲ）技术检测ＩｇＨ、ＴＣＲβ、ＴＣＲδ和ＴＣＲγ基因重排。结果在ＢＮＨＬ中，ＩｇＨ、ＴＣＲβ、ＴＣＲδ和ＴＣＲγ基因重排的检出结果分别为１０／１３（７７％）例、１３／１３（１００％）例、４／１３（３１％）例和８／１３（６２％）例；在ＴＮＨＬ中，上述不同基因重排的检出结果分别为３／１１（２７％）例、１０／１１（９１％）例、３／１１（２７％）例和３／１１（２７％）例。在１３例ＢＮＨＬ中，用ＴＣＲγ和ＴＣＲβ中的Ｄ１Ｊ２引物组合至少可检出有单一条带的有１１例（８５％），再加ＩｇＨ引物时可达１３例（１００％）。而在１１例ＴＮＨＬ中，用ＴＣＲγ和ＴＣＲβ中的Ｄ２Ｊ２引物组合至少可检出单一条带的有８例（７３％），再增加其他引物，不能显著提高单一条带的检出率。结论可用ＴＣＲγ和ＴＣＲβＤ１Ｊ１基因做为ＢＮＨＬ的ＭＲＤ检测标记，必要时加用ＩｇＨ基因重排；选用ＴＣＲγ和ＴＣＲβＤ２Ｊ２基因?

免疫球蛋白重链和T细胞受体γ基因重排在非霍奇金淋巴瘤中检测的临床意义

目的 :探讨免疫球蛋白重链 ( Ig H)和 T细胞受体 γ( TCRγ)基因重排在非霍奇金淋巴瘤( NHL )中的检测意义。方法 :用 PCR方法检测 2 5例 NHL和 1例反应性淋巴结炎患者 ,及 2 0例正常人骨髓、周围血和 /或淋巴结单个核细胞 ( MNCs)中克隆性 Ig H、TCRγ基因重排。结果 :克隆性Ig H和 /或 TCRγ基因重排在 2 5例 NHL 中检出为 84.0 % ( 2 1 / 2 5 ) ;克隆性 Ig H基因重排在 B-NHL和 T-NHL中检出分别为 86.7% ( 1 3 / 1 5 )和 2 0 .0 % ( 2 / 1 0 ) ,克隆性 TCRγ基因重排分别为5 3 .3 % ( 8/ 1 5 )和 80 .0 % ( 8/ 1 0 )。 1例反应性淋巴结炎和 2 0例正常人均未检测到 Ig H和 TCRγ基因重排。结论 :Ig H、TCRγ基因重排检测有助于 NHL 的诊断和鉴别诊断 ,及发现 NHL

15例急性淋巴细胞性白血病微小残留病追踪检测结果分析

为探讨残留白血病细胞的存在与白血病患儿长期生存之间的关系,我们用非同位素的PCR-RNA转录本分子杂交法,选用T细胞抗原受体γ链(TCR_γ)重排基因为标志,检测了20例急性淋巴细胞白血病(ALL)患儿,并对其中具有TCR_γ重排基因的15例患儿进行了追踪检测,结果显示:化疗后早期(<5月)大多数患儿都能检测到残留白血病细胞,长期缓解者微小残留病检测为阴性。结果表明,当临床达到完全缓解时,对每1例患者的残留白血病细胞进行监测是必要的。

一例AML中一种新的TCRδ基因重排及其分析方法

Ｔ细胞抗原受体（ＴＣＲ）功能的表达有赖于该基因在正常Ｔ淋巴细胞发育过程中的重排。近年来，已发现一些肿瘤及白血病中出现该基因的异常重排。我们采用聚合酶链反应（ＰＣＲ）、“磁珠”固相纯化方法和ＰＣＲ产物直接测序等方法，从一例ＡＭＬ中发现了一种在白血病中未报道过的ＴＣＲδ基因重排．该重排是一种新报道的Ｄδ区ＤδＸ片段的重排．为ＤδＸＤδ２Ｄδ３Ｊδ１不完全重排。在研究白血病ＴＣＲ基因重排中，采用本文所报道的方法，有助于新的重排的发现。

肝脾T细胞淋巴瘤13例临床病理分析及预后

目的探讨肝脾T细胞淋巴瘤(HSTCL)的临床病理学特点、诊断及鉴别诊断。方法收集13例HSTCL的临床资料并进行形态学观察,应用免疫组化和TCR基因重排检测,并复习相关文献。结果13例瘤细胞CD2、CD3、CD7均阳性,T细胞限制性胞内抗原TIA-1、CD56部分阳性,细胞毒性相关分子粒酶B(Granzyme-B)、EBER阴性。11例标本TCR克隆性重排检测阳性。13例患者临床治疗方案不同(脾切除术后化疗,保脾化疗,自体造血干细胞移植),随访6~58个月,预后均较差。结论HSTCL是一类罕见的结外侵袭性外周T细胞淋巴瘤,其病理表现多样且独特,结合免疫表型、TCR基因重排可确诊。

降落式PCR和SSCP检测淋巴细胞白血病单克隆T细胞受体γ基因重排

目的以降落式PCR和单链构型多态性(SSCP)方法检测淋巴细胞白血病单克隆T细胞受体(TCR)γ基因重排,探讨其在淋巴细胞白血病诊断中的价值。方法盐析法提取淋巴细胞白血病患者外周血白细胞DNA,TCR-γ基因重排通用引物和降落式PCR扩增基因重排。分别采用琼脂糖凝胶电泳、SSCP和DNA直接测序方法检测PCR扩增产物。阳性细胞系DNA模板与反应增生性淋巴组织DNA按不同比例混合后扩增,检测降落式PCR的灵敏度。结果琼脂糖电泳中,18例T淋巴细胞白血病中有15例、4例B淋巴细胞白血病中有2例为阳性,阳性标本经SSCP进一步分析,呈不连续条带。DNA直接测序证实扩增产物为TCR-γ基因重排。阳性对照模板占1%以上时可得到阳性扩增结果。结论TCR-γ基因重排通用引物结合降落式PCR可有效扩增T淋巴细胞白血病基因重排,可用于T淋巴细胞白血病的辅助诊断。

急性粒细胞白血病TCRγ基因重排的检测及其意义

①目的 探讨急性粒细胞白血病 (AML)中T细胞抗原受体γ链 (TCRγ)基因重排的发生情况及其与AML临床特征的关系。②方法 以构建的TCRγ基因片断为内参照模板 ,用聚合酶链反应 (PCR)法扩增TCRγ基因重排片断。③结果 TCRγ基因重排在AML中发生率为 2 4 .4 % ,在急性单核系白血病中发生率高达 4 8.1% ,差异有极显著性 (χ2 =12 .32 ,P <0 .0 0 1)。有TCRγ基因重排的AML病人的外周血白细胞计数高于无TCRγ基因重排的AML病人 (t=2 .5 35 ,P <0 .0 5 ) ;有TCRγ基因重排的AML病人的肝大程度大于无TCRγ基因重排的AML病人 (t=2 .35 7,P <0 .0 5 ) ;TCRγ基因重排阳性的AML病人达到第 1次缓解的时间长于TCRγ基因重排阴性的AML病人 (t=2 .5 32 ,P <0 .0 5 )。④结论 TCRγ基因重排可发生于部分髓系白血病病人 ,急性单核系白血病的发生率最高 ,这部分病人临床体征明显 ,对标准化疗不敏感 ,不易获得缓解。

中线T细胞淋巴瘤的TCR-γ基因重排研究

目的:对中线T细胞淋巴瘤的克隆性进行研究。方法:用一组针对T细胞受体γ链基因V区片段的家族特异性引物和PCR方法,对11例(22个标本)中线T细胞淋巴瘤病例进行了T细胞受体丁基因重排的检测。结果:22个标本中21个有T细胞受体γ链基因的克隆性重排(94.45％)。在9例原发灶的连续活检和1例原发灶及其转移灶的标本中均未发现增生的克隆家族的改变。结论:中线T细胞淋巴瘤的病变组织中存在T细胞的单克隆性增生,为该肿瘤的T细胞起源提供了分子生物学的证据。在中线T细胞淋巴瘤的疾病过程中(包括转移灶)增生T细胞的家族未发生变化,支持肿瘤的单克隆起源学说。

半重叠式多重引物PCR和基因扫描技术在T细胞淋巴瘤诊断中的应用

[目的]探讨半重叠式多重荧光多重引物PCR和基因扫描技术在T细胞淋巴瘤诊断中的应用.[方法]从普通石蜡切片组织标本中提取基因组DNA,用半重叠式多重荧光多重引物PCR扩增,利用DNA测序仪对其产物进行基因扫描分析.[结果]37例T细胞淋巴瘤中27例检测出有克隆性重排;25例B细胞淋巴瘤中2例呈阳性;10例何杰金氏淋巴瘤和7例反应性增生病例均呈阴性.[结论]在T细胞受体γ基因重排克隆性检测中,半重叠式多重荧光多重引物PCR及基因扫描技术具有样本来源便利,灵敏度高,特异性强,耗时短等优点,可作为T细胞淋巴瘤的诊断及鉴别诊断的辅助检测手段.

TCRγV_1/pcDNA3重组质粒的构建

目的:构建含TCRγV1重排基因的真核表达质粒。方法:从人淋巴瘤Jurkat细胞中提取mRNA,用RT-PCR法扩增含BamH与Hind酶切位点TCRγV1基因序列,对pcDNA3载体及TCRγV1基因PCR产物经双酶切,用连接酶将两者连接并转化到大肠杆菌DH5a,对重组质粒经序列测定,称pcDNA3/TCRγV1。结果:电泳获得333bp的TCRγV1预期条带。结论:该条带测序证实为TCRγV1基因序列。

抗原受体基因重排克隆性检测在淋巴瘤诊断中的应用

本研究旨在探讨抗原受体基因重排克隆性检测在淋巴瘤诊断中的意义。收集分析了31例淋巴瘤组织,石蜡包埋切片,HE染色后观察形态,免疫组织化学分析免疫表型。采用BIOMED-2标准化试剂盒检测抗原受体基因重排克隆性。结果表明,31例病例中形态学及免疫组织化学分析疑似T细胞淋巴瘤12例,T细胞反应性增生1例,B细胞淋巴瘤16例,B细胞反应性增生2例。基因重排克隆性检测免疫球蛋白(Ig)阳性率94.44%(17/18),T细胞抗原受体(TCR)阳性率92.31%(12/13),2例阴性。最终12例确诊为T细胞淋巴瘤,B细胞淋巴瘤17例,反应性增生2例,阳性检出率为93%。结论:抗原受体重排基因克隆性分析是诊断淋巴瘤的一种有效辅助手段。

PCR扩增TCR_γ基因重排检测急性淋巴细胞白血病微量残留病的研究

应用多聚酶链反应（ＰＣＲ）技术检测急性淋巴细胞白血病（ＡＬＬ）骨髓白血病细胞ＴＣＲγ基因重排，敏感性达１０￣（－５）水平以上。２７例急性期ＡＬＬ有２１例检测到约４００ｂｐ的扩增产物，阳性检出率为７７．８％（２１／２７）；７例完全缓解（ＣＲ）的ＡＬＬ有２例检测阳性，其中１例于检测后１．５月复发，另１例随访６个月仍ＣＲ；而其余５例检测阴性者于检测后平均随访７．１月均持续ＣＲ。提示本法对ＡＬＬＴＣＲ＿γ基因重排的检测较具普遍性，可用于其微量残留病（ＭＲＤ）的检测，对ＡＬＬ预后的判断、复发的监测可能有重要意义。

BIOMED-2系统应用于B细胞非霍奇金淋巴瘤抗原受体基因重排检测的研究

目的:探讨BIOMED-2系统在检测B细胞非霍奇金淋巴瘤中的应用价值。方法:选取石蜡包埋组织B细胞非霍奇金淋巴瘤40例、其他淋巴结增生性病变10例,提取组织DNA,应用BIOMED-2系统中的61条引物分成9个组别进行PCR扩增,检测DNA质量及抗原受体基因重排克隆性。结果:94%(47/50)样本DNA长度在300 bp以上,BIOMED-2系统检测的敏感性和特异性均为100%,Ig H-A、Ig H-B、Ig H-C、Ig H-D、Ig H-E、Ig K-A、Ig K-B、Ig L组检出率分别为45%(18/40)、27.5%(11/40)、87.5%(35/40)、55%(22/40)、47.5%(19/40)、80%(32/40)、50%(20/40)、22.5%(9/40),Ig H-C联合Ig K-A组合检出率为100%。结论:BIOMED-2系统适用于石蜡包埋组织B细胞抗原受体基因重排检测,具有很高的敏感性和特异性。

多发性硬化患者外周血T淋巴细胞受体β链可变区多态性研究

目的探讨多发性硬化(MS)不同阶段外周血T淋巴细胞受体β链可变区(TCRVβ)多态性的特点。方法收集首都医科大学宣武医院神经内科临床孤立综合征(CIS)患者30例、复发-缓解型多发性硬化(RRMS)患者40例、继发-进展型多发性硬化(SPMS)患者10例、健康对照者30名,经TCRVβ单克隆抗体标记后采用流式细胞仪分析各组外周血TCRVβ扩增程度以及TCRVβ24个亚家族扩增患者百分比、扩增片段所占百分比的差异。结果 CIS、RRMS及SPMS组TCRVβ存在扩增患者比例、扩增个数和扩增分数均高于对照组(P<0.01),而CIS、RRMS及SPMS组间比较无统计学差异(P>0.05)。CIS、RRMS及SPMS组CD4+TCRVβ2扩增频率均高于对照组(P<0.008),CIS组、RRMS及SPMS组CD8+TCRVβ11表达水平均低于对照组(P<0.05),SPMS组CD4+TCRVβ21.3表达水平低于CIS组(P<0.05)。ROC曲线分析提示CD8+TCRVβ11的扩增片段所占百分比对MS诊断具有一定价值,对MS分型无诊断价值;CD4+TCRVβ21.3的扩增片段所占百分比对SPMS诊断具有一定价值。结论可通过检测部分TCRVβ片段对MS及SPMS的早期诊断提供相关依据。

IgH/TCR基因重排与EB病毒原位杂交联合分析在淋巴瘤诊断中的应用

目的探讨免疫球蛋白重链/T细胞受体(IgH/TCR)基因重排检测联合EB病毒(EBV)原位杂交在淋巴瘤诊断中的应用,分析EBV+-B细胞淋巴瘤的细胞学及基因组学特征、鉴别诊断要点,以缩短诊断时间,减少误诊。方法采用IgH/TCR基因重排与EB原位杂交联合分析诊断EBV+-B细胞淋巴瘤1例,分析其免疫组化特征、EBV原位杂交、基因重排结果。结果 EBV+-B细胞淋巴瘤临床上主要表现为淋巴结增大,常伴骨髓和外周血浸润。淋巴结活检显示其结构破坏,淋巴滤泡减少,淋巴结高度增生性病变,可见轻至中度异型淋巴细胞,淋巴窦扩张,组织细胞增生。免疫组化证实EBV感染的细胞毒性B细胞构成病变主体;EBV原位杂交显示部分淋巴细胞核阳性;基因重排提示IgH、免疫球蛋白轻链(Igκ)基因发生克隆性重排,TCRγ无克隆性重排。结论 EBV+-B细胞淋巴瘤从形态学上难以与伯基特淋巴瘤、慢性淋巴细胞白血病等淋巴瘤区分,早期诊断困难。联合应用IgH/TCR基因重排与EBV原位杂交技术对EBV+-B细胞淋巴瘤的诊断有较高准确性。

Features of intestinal T-cell lymphomas in Chinese population without evidence of celiac disease and their close association with Epstein-Barr virus infection

Background Intestinal T-cell lymphoma （ITCL） is a heterogeneous lymphoid neoplastic group with variable clinical and pathological features. ITCL in oriental countries is different from enteropathy-type intestinal T-cell lymphoma （ETCL） in relation to celiac disease and Epstein-Barr virus （EBV）. The objective of this study was to investigate the clinicopathological features, immunophenotype, expression of cytotoxic molecule （TIA-1）, T-cell receptor （TCR）-γ gene rearrangement, and Epstein-Barr virus （EBV） latent infection in primary ITCL without celiac disease in Chinese. Methods The clinical data of 42 patients were analyzed, and the patients were followed up. Compared with human reactive lymphoid tissues, in situ hybridization for EBER1/2, polymerase chain reaction for TCR-~/gene rearrangement, and immunohistochemical staining for immunophenotypes, TIA-1 and EBV latent membrane proteins （LMP-1） were investigated. Survival curves of different clinicopathological features, immunophenotypes, expression of LMPI , TCR-γ/gene rearrangement and therapy were analyzed. Results Three fourths of the patients suffered from ITCL in China were men with a peak age incidence in the 4th decade. Common presenting features included fever and hemotochezia. The prognosis was poor with a median survival of 3.0 months. The lesions were mostly localized in the ileocecum and colon. About 38/42 （90. 5% ） patients demonstrated pleomorphic medium-sized on large seen. All 42 patients with ITCL revealed CD45RO cells. Histological features of celiac disease were rarely positive. Neoplastic cells partially expressed T-cell differentiated antigens （CD3ε, CD4, CD8） and NK cell associated antigen （CD56）. The positive frequency of CD3e, CIM, CD8 and CD56 was 28/42 （66.7%） 7/42 （16.7%）, 10/42 （23.8%） and 12/42 （28.6%） respectively. Thirty-nine cells （92. 9% ） expressed TIA-1, but none expressed CD20 and CD68. More than half of the patients （64. 3% , 64.3% and 59.5% ） revealed TCR-γ primers respectively. EBER1/2 was detected in 41 （97.6%） of LMP-1 was 38. 1% （16/42）. gene rearrangement by three different TCR-γ the 42 patients. The expression frequency ofConclusions Primary ITCL without celiac disease in Chinese is a special highly EBV-associated clinicopathological entity. There are few similarities in patients with celiac disease in western countries. A small proportion of primary ITCLs in Chinese and extranodal NK/T-eell lymphoma of nasal type belong to the same speetrum.