T-CELL RECEPTOR GENE REARRANGEMENT ANALYSIS IN THE PRIMARY CUTANEOUS T-CELL LYMPHOMA

Object: The present paper is to evaluate the significance of T cell receptor (TCR) gene rearrange ments in primary cutaneous T cell lymphomas (PCTCL) as detected by analysis of Southern Blot (SBA) and polymerase chain reaction (PCR). Patients and Methods: Skin specimens and peripheral blood samples were taken from 44 patients with PCTCL, including 30 patients with mycosis fungoides (MF), 2 patients with Sezary's syndrome (SS), and 12 patients with PCTCL other than MF and SS (PNCTCL). 11 patients with a presumptive diagnosis of MF, 23 patients with lymphoproliferative dermatoses including lymphomatoid papulosis (LyP) and 8 patients with benign cutaneous lymphoid infiltrates were simultaneously studied by the amplification of junctional V (variable) J (joining) sequences of the rearranged TCRγ genes by PCR(TCRγPCR) and the analysis of TCRb chain genes by SBA(TCRβSBA) for detection of clonal gene rearrangements (GR). One lymph node specimen of a case with MF IIA was also detected by TCRγ PCR and TCRβSBA. Results: In MF, GR were detected by TCRγPCR and TCRβSBAb in 83.3 85.7% and 66.7% 71.4% of skin specimens of cases IIA IIB and in 57.1% 70.0% and 14.3% 10.0% of those of cases IA IB, respectively. GR were seen in 66.7% 71.4% and 33.3% 43.0.% of blood samples of cases IIA IIB, and 42.9% 40.0% and 0 10.0% of those of cases IA IB, respectively. GR was confirmed by TCRγ PCR and TCRβSBA in one lymph node showing dermato pathic lymphadenopathy of a case with MF IIA. In 11 patients of clinically suspected MF, GR were present in skin specimens of 5 cases (45.4%) and in blood samples of 3 cases ( 27.3% ) by TCRγ PCR. In PNCTCL, GR were found in 9 skin specimens (90.0%) from 10 patients detected by TCRγ PCR and in 6 skin specimens (75.0%) from 8 patients detected by TCRβSBA. GR were also seen in 6 blood samples (72.8%) from 11 patients detected by TCRγ PCR, and in 7 blood samples (70.0%) from 10 patients by TCRβSBA. In SS and LyP, GR were detected by TCRγ PCR and TCRβSBA in each of the two skin specimens of two cases with LyP and in each of the two blood samples of two cases with SS. GR were seen in one skin specimen of one case with SS and one blood sample of one case with LyP detected by TCRγPCR. Conclusions: This study demonstrated that TCRγ PCR is a rapid, more sensitive tool than TCRβSBA, can be used in the analysis of T cell clonality in skin, lymph node and blood samples of patients with PCTCL and indicated that this method forms a useful supplement to other methods for diagnosis of early and suspected MF, confirmation of PNCTCL and determination of extracutaneous involvement of lymph node and blood.

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.

Diagnostic significance of TCR gene clonal rearrangement analysis in early mycosis fungoides

Mycosis fungoides(MF),the most common type of cutaneous T-cell lymphoma,has various unspecific clinical and histological characteristics.Its early diagnosis is challenging.The application of T-cell receptor(TCR) gene clonal rearrangement to the diagnosis of MF has been widely studied.In this study,we used polymerase chain reaction(PCR) to investigate the diagnostic significance of detecting TCR-γ and-β gene clonal rearrangement in the early diagnosis of mycosis fungoides.PCR for TCR-γ and TCR-β gene rearrangement was performed on 19 patients with suspected early MF,6 with typical MF,and 6 with chronic dermatitis.Of the 19 patients with suspected early MF,13 had TCR-γ gene clonal rearrangement,whereas none had TCR-β gene clonal rearrangement.All patients with typical MF had TCR gene clonal rearrangement,in which 4 showed TCR-γ clonal rearrangement,1 showed TCR-β gene clonal rearrangements,and 1 showed both.No patients with chronic dermatitis had TCR gene clonal rearrangement.These results indicate that TCR gene clonal rearrangement analysis is a useful tool in diagnosing early MF.TCR-γ gene is recommended to the routine analysis,whereas TCR-β gene has potential in combination toward intractable cases.

PCR-SSCP检测非霍奇金淋巴瘤患者骨髓克隆性T细胞受体基因重排及其临床意义

背景与目的:进一步了解非霍奇金淋巴瘤(non-Hodgkinslymphoma,NHL)患者骨髓标本克隆T细胞受体(Tcellreceptor,TCR)基因重排情况及临床意义。方法:应用聚合酶链反应(polymerasechainreaction,PCR)联合单链构象多态性(single-strandconformationpolymorphism,SSCP)分析43例NHL患者骨髓标本TCRVγI-Jγ基因重排情况。结果:43例NHL患者有26例(60.5%)存在克隆性TCRVγI-Jγ基因重排。16例骨髓形态学检查未发现淋巴瘤细胞浸润者中有3例(18.8%)发现克隆性TCRVγI-Jγ基因重排,此3例患者分别于4～9个月后行骨髓形态检查时发现淋巴瘤细胞浸润;27例骨髓形态学检查有淋巴瘤细胞浸润者有23例(85.2%)存在克隆性TCRVγI-Jγ基因重排阳性。26例PCR扩增阳性病例经SSCP分析发现7例(26.9%)存在寡/亚克隆重排。7例存在寡/亚克隆重排患者经3～11个月有5例(71.4%)发展为白血病,存在寡/亚克隆重排NHL患者1年内转化为白血病的发生率显著高于无寡/亚克隆重排患者(10.5%)(P<0.005)。结论:应用PCR检测NHL患者骨髓标本克隆性TCRVγI-Jγ基因重排可较骨髓形态学检查更早发现NHL患者骨髓浸润微小病灶。具有寡/亚克隆NHL患者更易发展为白血病,还可发展为急性非淋巴细胞白血病。

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.

原发性皮肤间变性大细胞淋巴瘤T细胞γ受体、IgH基因重排

目的:探讨原发性皮肤间变性大细胞淋巴瘤(C-ALCL)临床病理特点和基因诊断方法。方法:对6例C-ALCL的临床表现、病理形态学和免疫组化染色进行观察,并用PCR方法对石蜡标本进行T细胞γ受体(TCRγ)和重链免疫球蛋白(IgH)基因重排检测。结果:临床起病以孤立性结节多见,病情进展缓慢,个别可自行消退。5例患者经治疗病情稳定,1例死于淋巴结及肝脏转移。镜下以75%以上CD30+间变性大细胞弥漫浸润真皮及皮下脂肪组织为特点,多数瘤细胞表达T细胞免疫表型。5例标本TCRγ基因重排阳性。结论:C-ALCL是少见的原发皮肤的低度恶性T细胞性淋巴瘤,预后较好。综合临床表现、组织病理改变、免疫组化及基因重排检测有助于本病的正确诊断。

活动性肺结核患者α/βTCR基因重排及CDR3谱型分析

目的:建立多重PCR方法扩增α/βTCR全长序列,分析活动性肺结核患者病变局部T淋巴细胞α/βTCR基因重排特点及CDR3谱型。方法:分离结核患者肺泡灌洗液中的淋巴细胞,提取RNA后用SMART方法逆转录,运用根据现有文献设计的α和βTCR扩增引物,进行多重PCR扩增以获得其全长序列,构建重组质粒并测序,利用DNAstar及网上TCR资源分析序列。结果:3例患者共获得24个α链序列,13个β链序列。α链以AV1S2(54%)、AV12S3(41%)、AV12S2(5%)为主;β链以BV2(38%)、BV29S1(46%)、BV14(3%)、BV4S2(3%)为主。同一病例及不同病例之间CDR3区呈现多样性,但是标本1、标本3各有一条β链的CDR3氨基酸序列相同:SVGTGTLHQETQY;标本2和标本3的各有2条α链CDR3序列相同:AVRDWAGNMLT;标本2的一个α链和标本3的一个α链的CDR3均有:AV…DNN…RLM序列。结论:建立了TCRα和β链全长序列的多重PCR扩增方法。结核患者病变局部克隆性增殖的TCRα和β链谱型呈限制性取用,克隆增生的T淋巴细胞来自不同的亚群,但是相同的CDR3序列对于识别MTB多肽可能具有特异性。

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。

皮肤T细胞淋巴瘤皮损与外周血中TCRγ基因重排的检测

目的:了解已确诊为皮肤T细胞淋巴瘤(CTCL)患者的皮损和外周血中T细胞受体γ链基因重排(TCRγGR)情况。方法:利用PCR测定21例CTCL患者皮损及外周血TCRγGR,扩增产物经琼脂糖及变性梯度凝胶电泳检测。结果:CTCL患者皮损中TCRγGR阳性率显著高于外周血(P<0.05);病程≥12个月的患者外周血中TCRγGR阳性率显著高于病程<12个月的患者(P<0.05);年龄≥60岁患者皮损和外周血中TCRγGR阳性率显著高于<60岁患者(P<0.05)。结论:在CTCL患者中存在TCRγGR,早期出现在皮损中的TCRγGR可作为CTCL辅助诊断,并有益于CTCL的早期诊断,外周血中检测出TCRγGR可作为皮损阳性结果的补充。

琼脂糖凝胶电泳及SSCP法在淋巴瘤克隆性TCRγ基因重排检测中的应用

目的比较琼脂糖凝胶电泳和单链构象多态性分析(SSCP)法对淋巴瘤克隆性T细胞受体(TCR)γ基因重排的检测结果,探讨TCRγ基因重排的有效检测方法。方法从T、B细胞淋巴瘤及反应增生性淋巴组织中提取DNA,分别用两组TCRγ基因重排通用引物进行PCR扩增,扩增产物分别进行琼脂糖凝胶电泳和SSCP。结果T、B细胞淋巴瘤均出现克隆性TCRγ基因重排。SSCP法两组PCR产物在T细胞淋巴瘤中的阳性率分别为77.6%和75.9%,B细胞淋巴瘤均为10%;与SSCP相比,琼脂糖凝胶电泳中两组PCR扩增产物的假阳性率分别为15.3%和14.4%,所有反应增生性淋巴组织均出现假阳性。结论T、B细胞淋巴瘤中都存在克隆性TCRγ基因重排,仅用琼脂糖凝胶电泳检测可能出现假阳性,SSCP灵敏性较高。

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

2种电泳在淋巴瘤TCR-γ基因重排研究中的应用

目的 探讨不同电泳方法在淋巴瘤T细胞受体γ(TCR γ)基因重排研究中的应用及其意义。方法 在聚合酶链式反应 (PCR )中采用T细胞受体γ基因重排通用引物 ,对 3 0例T细胞淋巴瘤和 3 0例B细胞淋巴瘤组织扩增 ,并采用琼脂糖凝胶电泳和单链构型多态性分析实验对扩增产物进行研究。结果 2 9例T细胞淋巴瘤扩增产物在琼脂糖电泳中为阳性 ,其中 2 7例在SSCP分析实验中为阳性。 16例B细胞淋巴瘤在琼脂糖电泳中为阳性 ,其中 3例在SSCP分析实验中阳性。所有在琼脂糖电泳中阴性的PCR产物在SSCP分析实验中也为阴性。在琼脂糖电泳中真阳性与假阳性条带有差异。结论 在TCR γ基因重排扩增产物分析中 ,琼脂糖凝胶电泳可能产生假阳性结果 ,但无假阴性 ;琼脂糖凝胶电泳中的假阳性可在SSCP实验中排除。 2种电泳方法同时应用 ,可以减少工作量 。

N-甲基亚硝基脲诱导小鼠胸腺淋巴瘤TCR基因重排分析

目的探讨N-甲基亚硝基脲(MNU)诱导的小鼠胸腺淋巴瘤的单克隆起源。方法采用巢式PCR方法,对8例MNU诱导的胸腺淋巴瘤组织进行T细胞受体β链(TCRβ)和γ链(TCRγ)克隆性基因重排分析,并对TCRγ基因重排的PCR产物直接测序。结果 8例胸腺淋巴瘤检测TCRβ和TCRγ均呈克隆性基因重排。DNA序列测定证实TCRγ基因PCR扩增产物为基因重排产物。结论巢式PCR TCR基因重排检测及DNA序列分析证实,MNU诱导的小鼠胸腺淋巴瘤是来源于T细胞的肿瘤。

TCR基因重排在皮肤T细胞淋巴瘤中的应用

T细胞在成熟过程中通过T细胞表面受体基因重排,从而具有特异性识别抗原的能力,在这一过程中的任何失调都会导致疾病。皮肤T细胞淋巴瘤是由于单个淋巴细胞的恶性增殖所导致的,病变组织表现出T细胞受体基因重排克隆性。蕈样肉样肿和Sézary综合征为最常见的皮肤T细胞淋巴瘤。T细胞受体基因重排的检测在皮肤T细胞淋巴瘤的发病机制研究、分类、诊断、判断预后上有重要的作用。

T细胞淋巴瘤T细胞受体γ链基因重排的检测

目的 探讨T细胞淋巴瘤T细胞受体γ链基因重排的情况。方法 用免疫组化标记筛选 30例T细胞淋巴瘤、2例高度可疑为T细胞淋巴瘤和 10例淋巴结反应性增生 ,采用聚合酶链式反应扩增方法检测T细胞受体γ链基因重排。结果 30例T细胞淋巴瘤中 2 7例和 2例高度可疑为T细胞淋巴瘤均出现T细胞受体γ链基因重排 ,10例淋巴结反应性增生均无T细胞受体γ链基因重排。结论 T细胞淋巴瘤病变中存在T细胞单克隆增生 ,支持肿瘤单克隆起源学说 ;T细胞受体γ链基因重排检测是区分T细胞淋巴瘤和淋巴结反应性增生的有效方法 ,且对T细胞淋巴瘤疑难病例的诊断有帮助。

皮下脂膜炎性T细胞性淋巴瘤的临床特征及分子生物学特点

目的 :对皮下脂膜炎性T细胞淋巴瘤 (SPTCL)的临床特征、病理、免疫表型及分子生物学特点进行研究。方法 :临床观察及实验室、病理检查研究SPTCL的临床、病理特点 ,免疫表型通过用LCA、CD3、UCHL、L2 6单抗进行石蜡免疫过氧化物酶染色、用αβTCR、γδTCR抗体进行冷冻切片免疫过氧化物酶的染色 ,用识别V1δ、V2δ 的抗体进行γδTCR亚型分析 ,PCR检测SPTCL患者TCR基因重排。结果 :7例SPTCL患者均有皮下结节、高热、体重下降 ,5例出现嗜血细胞综合征 ,7例SPTCL患者均有电介质、酸碱平衡失调及酶学检查的异常。 7例SPTCL患者的病理均在脂肪组织内见大量异型淋巴细胞浸润 ,均表达LCA、CD3、UCHL ,不表达L2 6。 4例SPTCL患者中有 3例表达γδTCR ,1例表达αβTCR ,3例γδTCR患者均表达V2 +δ ,4例有 3例出现TCRγ基因重排。结论 :SPTCL大多病情严重 ,肿瘤细胞来源于T细胞系的皮肤淋巴细胞组织相关的V2 +δ 细胞 ,可以出现TCRγ基因重排。

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。

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。

检测IgH和TCRγ基因重排对NHL分期参考价值的探讨

目的:探讨以IgH和TCRγ基因重排为标志对NHL患者临床分期的参考价值.方法:多聚酶链反应(PCR)技术结合限制性酶谱分析患者骨髓和淋巴结细胞DNA IgH和TCRγ基因重排的克隆性.结果:形态学无骨髓浸润的23例NHL患者发现6例(26.1%)具单克隆基因重排.结论:IgH和TCRγ基因重排作为分子标志对形态学检查不能确认骨髓浸润的NHL患者的分期诊断有一定参考价值.