CN111638359A - 检测小细胞肺癌患者外周血循环肿瘤细胞pd-l1基因突变的免疫荧光试剂盒及检测方法 - Google Patents
检测小细胞肺癌患者外周血循环肿瘤细胞pd-l1基因突变的免疫荧光试剂盒及检测方法 Download PDFInfo
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Abstract
本发明提供了一种检测小细胞肺癌患者外周血循环肿瘤细胞PD‑L1基因突变的免疫荧光试剂盒及检测方法,属于分子生物学技术领域。该试剂盒包括稀释液45mL、脱色液1mL、染色液A 0.5mL、染色液B 1mL、甲醇200μl、2%PFA 200μl、10%山羊血清100μl、一抗工作液100μl、二抗工作液100μl、DAPI封片剂。本发明提供的检测方法,不用穿刺活检获取组织标本即可检测到晚期或复发小细胞肺癌患者PD‑L1表达情况。该技术属于微创,并能够实时检测。本发明提供的方法,能够避免染色过程中可能产生的边缘效应导致的假阳性结果,稳定性好,降低细胞的损失,提高检测的准确性。
Description
技术领域
本发明提供了一种检测小细胞肺癌患者外周血循环肿瘤细胞PD-L1基因突变的免疫荧光试剂盒及检测方法,属于分子生物学技术领域。
背景技术
肺癌是导致癌症患者死亡的主要恶性肿瘤之一,在我国,肺癌的发病率和死亡率均居第一位。小细胞肺癌 (small cell lung cancer,SCLC)约 占肺癌发生率的15%~20%,相较非小细胞肺癌,具有更快的肿瘤倍增时间,快速生长以及易于早期转移的特点。
循环肿瘤细胞(Circulating tumor cell,CTC)是从实体肿瘤脱落进入外周血液循环的肿瘤细胞,自1989年被发现以来,目前已有多种方法用于外周血循环肿瘤细胞的检测。近期研究表明,其检测对于评估肿瘤患者尤其是晚期肿瘤患者的预后以及选择合适的个体化治疗具有重要的临床意义。因CTC检测具有微创、实时检测等特点,被称为肿瘤的“液态活检”。
目前,山东省第一医科大学、山东省药物研究院联合山东凯歌智能机器有限公司就循环肿瘤细胞检测鉴定关键技术、检测设备、试剂盒开发与生产进行合作,山东祺欣生物科技有限公司、山东喻晓生物科技有限公司、济南杏恩生物科技有限公司、山东发现生物技术有限公司等单位进行推广应用,本项目为山东省重大科技创新工程项目,以山东第一医科大学济南校区的山东省药物研究院为核心,落实注册人制度,依托循环肿瘤细胞检测鉴定核心诊断技术,进一步注册鉴定诊断试剂盒,以包括PD1、PD-L1、ER、PR、Her-2、GPC-3、VEGF、P53、Vimentin、TKI-EGFR、RAS、CK、ALK-D5F3、CD20、ALK/EML4、Beta-catenin、E-Cadherin、EP-CAM、HPV、IDH-1、PSA、PSMA、VEGF、GFAP、细胞角蛋白、AE1/AE3、雌激素受体、孕激素受体、BCA-225、CA 125、CEA、EMA、ERCC1、HPV、Ki-67、P53、TOP2A等作为CTCs表达的示踪剂,注册超灵敏、超快速、高覆盖、低成本、准确特异的鉴定诊断试剂盒,通过与在济南注册的山东凯歌智能机器有限公司、山东祺欣生物科技有限公司、山东喻晓生物科技有限公司、济南杏恩生物科技有限公司、山东发现生物技术有限公司合作进行研发与推广。
随着分子生物学的发展, PD-1/PD-L1为免疫靶点的免疫疗法为小细胞肺癌治疗带来了新的曙光。研究发现,免疫抑制与免疫逃逸和肿瘤细胞PD-L1的过表达密切相关,肿瘤细胞可通过其表面的PD-L1与免疫细胞T细胞表面的PD-1结合,传导抑制性信号,使得T细胞不能识别肿瘤细胞和向肿瘤细胞发出攻击信号,导致了肿瘤细胞免疫逃逸。基于此理论提出假设,自原发灶脱落进入循环系统的循环肿瘤细胞(CTC)出现凋亡、免疫清除或存活、转移结局与PD-L1表达密切相关。PD-1或PD-L1免疫制剂的疗效多与肿瘤组织中PD-L1的免疫组化表达水平有关,提示PD-L1表达水平可能是预测PD-1免疫治疗疗效的生物标志物;还有研究表明小细胞肺癌组织中PD-L1的高表达与肿瘤侵袭性呈正相关。因此,检测循环肿瘤细胞(CTC)PD-L1表达情况对小细胞肺癌预后及免疫治疗疗效评估具有重要价值。
发明内容
为了克服晚期或复发小细胞肺癌患者无法实时或反复穿刺获取组织标本、进而不能评估患者PD-L1状态的不足,本发明提供了一种小细胞肺癌患者外周血循环肿瘤细胞PD-L1基因突变非诊断目的的检测方法:利用膜过滤装置分离获得无法获取组织标本的晚期或复发小细胞肺癌患者外周血中的CTC,进一步运用免疫荧光技术检测CTC的PD-L1表达情况。
本发明采用的技术方案如下:
本发明提供了一种检测小细胞肺癌患者外周血循环肿瘤细胞PD-L1基因突变的免疫荧光试剂盒,包括稀释液45mL、、脱色液1mL、染色液A 0.5mL、染色液B 1mL、甲醇200μl、2% PFA200μl 、10%山羊血清100μl 、一抗工作液100μl、二抗工作液100μl、DAPI封片剂。
进一步的,所述一抗工作液是由小鼠抗CK、大鼠抗CD45和 兔抗PD-L1组成,分别采用BD wash buffer按1:100&1:500&1:400稀释混匀;所述二抗工作液是由荧光标记的小鼠抗羊、荧光标记的大鼠抗羊和荧光标记的兔抗羊组成,分别采用BD wash buffer按1:500稀释混匀。
进一步的,所述稀释液是由1mmol/L EDTA+0.1% BSA+0.1%海藻糖+0.2%聚氧乙烯聚氧丙烯醚嵌段共聚物组成,所述基础液为Tris-HCl缓冲剂。
进一步的,所述脱色液是由95%酒精与100%二甲苯按容积比1:1组成。
进一步的,所述染色液A为DAB染色液;所述染色液B为苏木素染色液。
本发明还提供了一种利用权利要求1-5任一项所述的免疫荧光试剂盒非诊断目的检测小细胞肺癌患者外周血循环肿瘤细胞PD-L1基因突变的方法,包括以下步骤:
(1)利用膜过滤装置分离获取无法获得组织标本的晚期或复发小细胞肺癌患者外周血中的CTC:采集无法获取组织标本的晚期或复发小细胞肺癌患者外周血:肘正中静脉外周血5ml;
(2)外周血样预处理:将采集的外周血样采用稀释液进行10倍稀释,稀释后加多聚甲醛固定外周血样10分钟,固定终浓度为0.25%;
(3)利用膜过滤分离肿瘤细胞装置过滤外周血样,分离获得外周血CTC:将预处理的外周血样加入到膜过滤分离肿瘤细胞装置的血样容器中,使其依靠重力自然过滤;
(4)过滤结束后,从膜过滤分离肿瘤细胞装置中取下滤器,将循环肿瘤细胞染色液A液0.5ml加入到滤器中,染色3min,PBS缓冲液冲洗干净;滤液过滤完全后加入染色液B液1ml,染色2min,纯水1ml冲洗2次,向滤器中加入200μl 2% PFA,室温固定5min,完成后0.5ml PBS漂洗3次,每次2min;再向滤器中加入200μl预冷的甲醇,4℃固定15min;取下滤膜,将滤膜下表面平整的贴附到载玻片一侧,将载玻片置于室温干燥4-5min后,使用镊子快速将滤膜从载玻片表面一次性揭起,转移至载玻片中央,滴加2ul贴片剂,干燥后在显微镜下观察,确定是否存在CTC;
(5)运用免疫荧光法检测CTC的PD-L1表达情况。
本发明免疫荧光检测CTC的PD-L1表达的具体方法如下:
(1)脱色:将带有CTC的滤膜从载玻片上取下,置于脱色液中浸泡4-6小时,脱去CTC染色液,PBS洗2min×3次;
(2)封闭:向滤膜上滴加100μl 10%山羊血清,室温放置30min,完成后吸去多余的血清;
(3)一抗孵育:弃掉载玻片上的封闭液,并立即滴加100μl一抗稀释液置于湿盒37℃孵育60min(或4℃过夜孵育,次日置于37℃复温30min);
(4)完成后PBS漂洗3次,每次3min;
(5)二抗孵育:滴加100μl二抗稀释液,室温孵育30min;
(6)完成后PBS漂洗3次,每次2min;
(7)使用含DAPI的封片剂封片,阅片,采图;
(8)采照完成后,脱片后进行瑞氏吉姆萨染色,与IF结果进行对比。
采图标准(对阳性细胞进行采图)
本发明所使用的膜过滤分离肿瘤细胞装置,包括滤器、血样容器、废液缸和铁架台,所述铁架台设有底座、立架和支架,所述血样容器通过支架设置于铁架台上部,血样容器的下方为滤器,滤器通过输液器联通至废液缸,废液缸设置于底座上。
所述滤器包括滤器上口、滤膜、载滤膜平台和滤器下口,滤膜置于载滤膜平台上;滤器上口接血样容器,滤器下口通过输液器接废液缸。
所述滤膜为疏水材料制成,其上均匀布满口径为8微米的滤孔。
本发明的有益效果是:
(1)本发明提供的检测方法,不用穿刺活检获取组织标本即可检测到晚期或复发小细胞肺癌患者PD-L1表达情况。该技术属于微创,并能够实时检测。
(2)本发明提供的方法,能够避免染色过程中可能产生的边缘效应导致的假阳性结果,稳定性好,降低细胞的损失,提高检测的准确性。
附图说明
图1为本发明的膜过滤装置结构示意图;
图2为本发明膜过滤装置的滤器的结构示意剖视图;
图3为本发明膜过滤装置的滤器滤膜的结构示意图;
图4 为晚期小细胞肺癌患者外周血循环肿瘤细胞PD-L1免疫荧光图像。
图中:1铁架台、2血样容器、3滤器、4输液器、5废液缸、6滤器上口、7滤膜、8载滤膜平台、9滤器下口、10滤孔、11底座、12立架、13支架。
具体实施方式
下面结合附图和实施例对本发明阐述如下。
本发明所使用的试剂盒具体规格如表1所示:
表1
运用此技术方法分离获取并鉴定10例非小细胞肺癌患者(同时检测10例正常人样本做阴性对照)外周血循环肿瘤细胞的实施例。
实施例1
一、利用膜过滤装置分离获取无法获得组织标本的晚期或复发小细胞肺癌患者外周血中的CTC,确定CTC是否存在:
自肘正中静脉采集空腹8-12小时的空腹血5ml,用45ml稀释液(成分:1mmol/L EDTA+0.1% BSA+0.1%海藻糖+0.2%聚氧乙烯聚氧丙烯醚嵌段共聚物)稀释外周血,然后加入3ml的4%多聚甲醛固定稀释后的血样10分钟;
在固定的间期,组装膜过滤装置:如附图1、图2、图3所示,该过滤装置由滤器3、滤膜7、血样容器2、废液缸5、铁架台1构成;
用10mlPBS润湿滤器3,然后将固定好的外周血样加入到膜过滤装置的血样容器2中,使其依靠重力自然过滤,CTC被截留在滤膜7上;
肿瘤细胞直径一般大于15微米,而血细胞(包括红细胞、白细胞)直径一般小于8微米,因此当含有CTC的外周血经过滤后,血细胞因直径小于滤孔10能够被滤过,而CTC因直径大于滤孔10被截留在滤膜7上。
过滤结束后,从过滤装置中取下滤器3,打开并移走滤器上口6,将将循环肿瘤细胞染色液A液0.5ml加入到滤器中,染色3min,PBS缓冲液冲洗干净;滤液过滤完全后加入B液,1ml,染色2min,纯水1ml,PBS缓冲液将滤器3冲洗干净,用眼科镊子取下滤膜7,细胞面朝上,放置在载玻片上;
将滤膜干燥后在显微镜下观察,确定是否存在CTC。
通过观察,10例健康志愿者均未查到CTC;除2例复发小细胞肺癌患者及1例晚期小细胞肺癌患者未检测到CTC外,其余7例均检测到CTC(表2),本次检测阳性率为70%,值得注意的是,当稀释液不添加0.1%海藻糖或者不添加0.2%聚氧乙烯聚氧丙烯醚嵌段共聚物时,单一的采用0.3%海藻糖或者0.3%聚氧乙烯聚氧丙烯醚嵌段共聚物,制备的血样稳定性差,部分血样还会形成分层,血液细胞容易发生聚集和粘连,影响最终的检测效果。
表2 实施例CTC检测结果
二、运用免疫荧光技术检测CTC的PD-L1表达情况:
(1)脱色:将带有CTC的滤膜从载玻片上取下,置于脱色液中浸泡4-6小时,脱去CTC染色液,PBS洗2min×3次;
(2)封闭:向滤膜上滴加100μl 10%山羊血清,室温放置30min,完成后吸去多余的血清(注:山羊血清采用用pH值为7.4的PBS缓冲液稀释);
(3)一抗孵育:弃掉载玻片上的封闭液,并立即滴加100μl一抗稀释液,一抗工作液是由小鼠抗CK、大鼠抗CD45和 兔抗PD-L1组成,分别采用BD wash buffer按1:100&1:500&1:400稀释混匀,置于湿盒37℃孵育60min(或4℃过夜孵育,次日置于37℃复温30min);
(4)完成后PBS漂洗3次,每次3min;
(5)二抗孵育:滴加100μl二抗稀释液,二抗工作液是由荧光标记的小鼠抗羊、荧光标记的大鼠抗羊和荧光标记的兔抗羊组成,分别采用BD wash buffer按1:500稀释混匀,室温孵育30min;
(6)完成后PBS漂洗3次,每次2min;
(7)使用含DAPI的封片剂封片,阅片,采图;
(8)采照完成后,脱片后进行瑞氏吉姆萨染色,与IF结果进行对比。
图4为晚期小细胞肺癌患者外周血循环肿瘤细胞免疫荧光染色图像,根据免疫学及形态学表现,发现肿瘤细胞细胞体积大,核质比异常,免疫学表现为典型的CTCs,其中,A为merge;B为CD45;C为PD-L1E;D为CK。
所检测的循环肿瘤细胞应用免疫组化证实PD-L1的表达并与小细胞肺癌大体标本PD-L1结果对比,观察其差异,主要针对大体标本PD-L1表达阴性而循环肿瘤细胞表达阳性的患者,指导小细胞肺癌的靶向治疗,为小细胞肺癌靶向治疗提供新的思路。
Claims (7)
1.一种检测小细胞肺癌患者外周血循环肿瘤细胞PD-L1基因突变的免疫荧光试剂盒,其特征在于,包括稀释液45mL、、脱色液1mL、染色液A 0.5mL、染色液B 1mL、甲醇200μl、2%PFA 200μl 、10%山羊血清100μl 、一抗工作液100μl、二抗工作液100μl、DAPI封片剂。
2.根据权利要求1所述的免疫荧光试剂盒,其特征在于,所述一抗工作液是由小鼠抗CK、大鼠抗CD45和 兔抗PD-L1组成,分别采用BD wash buffer按1:100&1:500&1:400稀释混匀;所述二抗工作液是由荧光标记的小鼠抗羊、荧光标记的大鼠抗羊和荧光标记的兔抗羊组成,分别采用BD wash buffer按1:500稀释混匀。
3.根据权利要求1所述的免疫荧光试剂盒,其特征在于,所述稀释液是由1mmol/L EDTA+0.1% BSA+0.1%海藻糖+0.2%聚氧乙烯聚氧丙烯醚嵌段共聚物组成,所述基础液为Tris-HCl缓冲剂。
4.根据权利要求1所述的免疫荧光试剂盒,其特征在于,所述脱色液是由95%酒精与100%二甲苯按容积比1:1组成。
5.根据权利要求1所述的免疫荧光试剂盒,其特征在于,所述染色液A为DAB染色液;所述染色液B为苏木素染色液。
6.一种利用权利要求1-5任一项所述的免疫荧光试剂盒非诊断目的检测小细胞肺癌患者外周血循环肿瘤细胞PD-L1基因突变的方法,其特征在于,包括以下步骤:
(1)利用膜过滤装置分离获取无法获得组织标本的晚期或复发小细胞肺癌患者外周血中的CTC:采集无法获取组织标本的晚期或复发小细胞肺癌患者外周血:肘正中静脉外周血5ml;
(2)外周血样预处理:将采集的外周血样采用稀释液进行10倍稀释,稀释后加多聚甲醛固定外周血样10分钟,固定终浓度为0.25%;
(3)利用膜过滤分离肿瘤细胞装置过滤外周血样,分离获得外周血CTC:将预处理的外周血样加入到膜过滤分离肿瘤细胞装置的血样容器中,使其依靠重力自然过滤;
(4)过滤结束后,从膜过滤分离肿瘤细胞装置中取下滤器,将循环肿瘤细胞染色液A液0.5ml加入到滤器中,染色3min,PBS缓冲液冲洗干净;滤液过滤完全后加入染色液B液1ml,染色2min,纯水1ml冲洗2次,向滤器中加入200μl 2% PFA,室温固定5min,完成后0.5ml PBS漂洗3次,每次2min;再向滤器中加入200μl预冷的甲醇,4℃固定15min;取下滤膜,将滤膜下表面平整的贴附到载玻片一侧,将载玻片置于室温干燥4-5min后,使用镊子快速将滤膜从载玻片表面一次性揭起,转移至载玻片中央,滴加2ul贴片剂,干燥后在显微镜下观察,确定是否存在CTC;
(5)运用免疫荧光法检测CTC的PD-L1表达情况。
7.根据权利要求6所述的方法,其特征在于,所述检测CTC的PD-L1表达的具体方法如下:
(1)脱色:将带有CTC的滤膜从载玻片上取下,置于脱色液中浸泡4-6小时,脱去CTC染色液,PBS洗2min×3次;
(2)封闭:向滤膜上滴加100μl 10%山羊血清,室温放置30min,完成后吸去多余的血清;
(3)一抗孵育:弃掉载玻片上的封闭液,并立即滴加100μl一抗稀释液置于湿盒37℃孵育60min(或4℃过夜孵育,次日置于37℃复温30min);
(4)完成后PBS漂洗3次,每次3min;
(5)二抗孵育:滴加100μl二抗稀释液,室温孵育30min;
(6)完成后PBS漂洗3次,每次2min;
(7)使用含DAPI的封片剂封片,阅片,采图;
(8)采照完成后,脱片后进行瑞氏吉姆萨染色,与IF结果进行对比。
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WO2021213322A1 (zh) * | 2020-04-21 | 2021-10-28 | 山东第一医科大学(山东省医学科学院) | 一种检测肾癌患者外周血循环肿瘤细胞pd-l1表达的免疫荧光试剂盒及检测方法 |
WO2021213262A1 (zh) * | 2020-04-20 | 2021-10-28 | 山东第一医科大学(山东省医学科学院) | 一种检测胃癌患者外周血循环肿瘤细胞pd-l1表达的免疫荧光试剂盒及检测方法 |
WO2021213299A1 (zh) * | 2020-04-20 | 2021-10-28 | 山东第一医科大学(山东省医学科学院) | 一种检测前列腺癌患者外周血循环肿瘤细胞pd-l1基因突变的试剂盒及检测方法 |
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Cited By (3)
Publication number | Priority date | Publication date | Assignee | Title |
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WO2021213262A1 (zh) * | 2020-04-20 | 2021-10-28 | 山东第一医科大学(山东省医学科学院) | 一种检测胃癌患者外周血循环肿瘤细胞pd-l1表达的免疫荧光试剂盒及检测方法 |
WO2021213299A1 (zh) * | 2020-04-20 | 2021-10-28 | 山东第一医科大学(山东省医学科学院) | 一种检测前列腺癌患者外周血循环肿瘤细胞pd-l1基因突变的试剂盒及检测方法 |
WO2021213322A1 (zh) * | 2020-04-21 | 2021-10-28 | 山东第一医科大学(山东省医学科学院) | 一种检测肾癌患者外周血循环肿瘤细胞pd-l1表达的免疫荧光试剂盒及检测方法 |
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