CN109485726B - 放射性标记抗纳米抗体在癌症的预后、诊断中的应用 - Google Patents
放射性标记抗纳米抗体在癌症的预后、诊断中的应用 Download PDFInfo
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Abstract
本发明公开了一种放射性标记抗纳米抗体在癌症的预后、诊断中的应用。具体地,本发明公开了一种用于检测PD‑L1分子的免疫偶联物,所述的免疫偶联物包含特定的抗PD‑L1纳米抗体的VHH链和放射性核素,可以用于待测对象PD‑L1表达情况的非侵入性检测。本发明的免疫偶联物具有小尺寸和高度特异性,适合同时靶向原发及转移肿瘤的全身检测,准确度高,辐射剂量小。
Description
技术领域
本发明涉及生物医学或生物显像技术领域,更具体地涉及放射性标记抗纳米抗体在癌症的预后、诊断中的应用。
背景技术
PD-1及其配体PD-L1是肿瘤免疫的重要靶点,利用单抗阻断PD-1、PD-L1通路近年受到人们广泛关注。PD-1、PD-L1是一对免疫抑制分子,是免疫系统防止自身免疫性疾病的重要组成部分,其通路的激活具有抑制肿瘤免疫应答、诱导肿瘤特异性T细胞凋亡的作用,与肿瘤发展有密切关系。PD-1(CD279)是一种 I型跨膜蛋白,属于免疫球蛋白超家族成员,主要表达于活化的CD4+T细胞、 CD8+T细胞及B细胞等免疫细胞上。其配体PD-L1(又名B7-H1,CD274)属于B7家族成员,在肿瘤浸润免疫细胞(TIC),以及多种恶性肿瘤细胞中高表达,如恶性黑色素瘤、非小细胞肺癌、头颈鳞癌等。在临床试验中,PD-1、PD-L1单抗显示出良好的疗效和安全性。美国FDA已批准多种抗PD-1、PD-L1单抗用于治疗黑色素瘤、非小细胞肺癌、晚期肾细胞癌等,还有多项PD-1、PD-L1单抗的临床试验正在进行中。
肿瘤通过上调PD-L1的表达,逃避机体免疫系统的识别与杀伤,临床标本证明PD-L1在多种恶性肿瘤组织及TIC上的高表达均与癌症患者的不良预后高度相关。虽然PD-1、PD-L1单抗在各种恶性肿瘤临床试验中显示出良好治疗效果,但是总体反应率只有大约20%,出现临床反应的肿瘤患者多为在治疗前TIC 或肿瘤细胞PD-L1高表达患者。因此各种PD-1、PD-L1单抗在肿瘤患者接受阻断治疗前,均须要对活检肿瘤组织检测PD-L1表达水平,以便对患者进行筛选,提高治疗临床效益。由于PD-L1是一个动态生物标志物,表达水平在治疗过程中随时间改变,传统组织穿刺检查方法在实践中有很多弊端。因此急需开发更有的效诊断方法,同时检测原发及转移肿瘤,实时及无创地检测及定量PD-L1 这一个动态生物标志物,筛选合适病人进行治疗,监测治疗效果及优化治疗方案。另外,PD-1、PD-L1单抗与局部放疗联合应用显示出较好的疗效,不但可以增强机体抗肿瘤免疫反应,还可产生远隔效应抑制远位肿瘤。利用抗体针对 PD-L1进行靶向性放疗,能够提高治疗效率及减少毒性,但目前这治疗模式尚处于起步阶段,其作用机制尚需进一步研究。
纳米抗体是目前最小的抗体分子,其分子量是普通抗体的1/10,最初由比利时科学家Hamers,R在骆驼血液中发现,它是工程化抗体产品中备受关注的一类。纳米抗体除具备单克隆抗体的抗原反应性外,还拥有一些独特的功能特性,如分子质量小,稳定性强、可溶性好、易表达、免疫原性弱(与人蛋白序列有超过70%相似)、穿透性强、靶向性强、人源化简单,制备成本低廉等,几乎完美克服了传统抗体开发周期长,稳定性较低,保存条件苛刻等缺陷。纳米抗体因其结构特殊,作为放射性同位素靶向载体,能够快速、特异性地穿透肿瘤组织结合靶标,而无结合抗体能很快从血液清除,减低身体放射性剂量,对比传统抗体作为示踪剂具有众多明显优势。
然而,目前本领域尚缺乏令人满意的针对PD-L1的纳米抗体。因此,本领域迫切需要开发新的有效针对PD-L1的特异性纳米抗体。
发明内容
本发明的目的在于提供一类有效针对PD-L1的特异性纳米抗体。
更具体的,本发明的目的在于提供针对于PD-L1的纳米抗体结合同位素标记非侵入性地检测PD-L1表达的应用。
在本发明的第一方面,提供了一种免疫偶联物,所述的免疫偶联物含有:
(a)抗PD-L1纳米抗体的VHH链或具有所述的VHH链的抗PD-L1纳米抗体,其中,所述的VHH链的氨基酸序列如SEQ ID NO.:1-7中任一所示;和
(b)选自下组的偶联部分:可检测标记物、药物、毒素、细胞因子、放射性核素、酶抗体、抗体Fc片段、抗体scFv片段、金纳米颗粒/纳米棒、病毒颗粒、脂质体、纳米磁粒、或细胞。
在另一优选例中,所述的偶联部分为放射性核素。
在另一优选例中,所述的放射性核素包括:
(i)诊断用同位素,所述的诊断用同位素选自下组:Tc-99m、Ga-68、F-18、 I-123、I-125、In-111、Ga-67、Cu-64、Zr-89、C-11、或其组合;和/或
(ii)治疗用同位素,所述的治疗用同位素选自下组Lu-177、Y-90、Ac-225、 As-211、Bi-212、Bi-213、Cs-137、Cr-51、Co-60、Dy-165、Er-169、Fm-255、Au-198、Ho-166、I-125、I-131、Ir-192、Fe-59、Pb-212、Mo-99、Pd-103、P-32、K-42、 Re-186、Re-188、Sm-153、Ra223、Ru-106、Na24、Sr89、Tb-149,、Th-227、Xe-133 Yb-169、Yb-177或其组合。
在另一优选例中,所述的药物为细胞毒性药物。
在另一优选例中,所述的细胞毒性药物选自下组:
抗微管蛋白药物、DNA小沟结合试剂、DNA复制抑制剂、烷化试剂、抗生素、叶酸拮抗物、抗代谢药物、化疗增敏剂、拓扑异构酶抑制剂、长春花生物碱等。
特别有用的细胞毒性药物类的例子包括,例如,DNA小沟结合试剂、DNA烷基化试剂、和微管蛋白抑制剂、典型的细胞毒性药物包括、例如奥瑞他汀(auristatins)、喜树碱(camptothecins)、多卡霉素/倍癌霉素(duocarmycins)、依托泊甙 (etoposides)、美登木素(maytansines)和美登素类化合物(maytansinoids)(例如 DM1和DM4)、紫杉烷(taxanes)、苯二氮卓类(benzodiazepines)或者含有苯二氮卓的药物(benzodiazepinecontaining drugs)(例如吡咯并[1,4]苯二氮卓类(PBDs),吲哚啉苯并二氮卓类(indolinobenzodiazepines)和噁唑烷并苯并二氮卓类(oxazolidinobenzodiazepines))、长春花生物碱(vinca alkaloids)、或其组合。
在另一优选例中,所述的毒素选自下组:
耳他汀类(例如,耳他汀E、耳他汀F、MMAE和MMAF)、金霉素、类美坦西醇、篦麻毒素、篦麻毒素A-链、考布他汀、多卡米星、多拉司他汀、阿霉素、柔红霉素、紫杉醇、顺铂、cc1065、溴化乙锭、丝裂霉素、依托泊甙、替诺泊甙(tenoposide)、长春新碱、长春碱、秋水仙素、二羟基炭疽菌素二酮、放线菌素、白喉毒素、假单胞菌外毒素(PE)A、PE40、相思豆毒素、相思豆毒素A链、蒴莲根毒素A链、α-八叠球菌、白树毒素、迈托毒素(mitogellin)、局限曲菌素(retstrictocin)、酚霉素、依诺霉素、麻疯树毒蛋白(curicin)、巴豆毒素、卡奇霉素、肥皂草(Sapaonaria officinalis)抑制剂、糖皮质激素、或其组合。
在另一优选例中,所述的免疫偶联物含有:多价(如二价)的所述VHH链或具有所述的VHH链的抗PD-L1纳米抗体。所述多价是指,在所述免疫偶联物的氨基酸序列中包含多个重复的所述VHH或所述的抗PD-L1纳米抗体。
在另一优选例中,所述的免疫偶联物用于癌症的预后、诊断中的PD-L1表达的检测。
在另一优选例中,所述的检测为体内检测。
在另一优选例中,所述免疫偶联物用于治疗或预防表达PD-L1蛋白(即PD-L1 阳性)的肿瘤。
在本发明的第二方面,提供了一种PD-L1蛋白检测试剂,所述的检测试剂包含本发明第一方面所述的免疫偶联物和检测学上可接受的载体。
在另一优选例中,所述的免疫偶联物的偶联部分为诊断用同位素。
在另一优选例中,所述的检测学上可接受的载体为无毒的、惰性的水性载体介质。
在另一优选例中,所述的检测试剂为选自下组的一种或多种试剂:同位素示踪剂、造影剂、流式检测试剂、细胞免疫荧光检测试剂、纳米磁粒和显像剂。
在另一优选例中,所述的检测试剂为造影剂,并且,所述的造影剂还包含用于造影的其他制剂。
在另一优选例中,所述的造影剂是用于MRI(磁共振成像)或CT(电子计算机X射线断层扫描技术)的造影剂。
在另一优选例中,所述的显像剂同时螯合了两种或多种信号,如Ga-68和Gd,同时用于PET/CT和MRI;或Tc-99m和荧光剂,同时用于SPECT/CT和荧光检测。
在另一优选例中,所述的检测试剂用于体内检测。
在另一优选例中,所述的检测试剂的剂型为液态或粉状(如水剂,针剂,冻干粉,片剂,含服剂,吸雾剂)。
在本发明的第三方面,提供了一种药物组合物,所述的包含本发明第一方面所述的免疫偶联物和药学上可接受的载体。
在另一优选例中,所述的免疫偶联物的偶联部分为药物、毒素、和/或治疗用同位素。
在另一优选例中,所述的药物组合物中还含有治疗肿瘤的其他药物,如细胞毒性药物。
在另一优选例中,所述的药物组合物用于治疗或预防表达PD-L1蛋白(即PD-L1 阳性)的肿瘤。
在另一优选例中,所述肿瘤包括:胃癌、淋巴瘤、肝癌、白血病、肾脏肿瘤、肺癌、小肠癌、骨癌、前列腺癌、结直肠癌、乳腺癌、大肠癌、前列腺癌、或肾上腺肿瘤。
在另一优选例中,所述的药物组合物为注射剂型。
在本发明的第四方面,提供了一种检测PD-L1分子的试剂盒,所述试剂盒含有本发明第一方面所述的免疫偶联物和说明书。
在另一优选例中,所述的说明书记载,所述的试剂盒用于非侵入性地检测待测对象的PD-L1表达。
在另一优选例中,所述的试剂盒用于表达PD-L1蛋白(即PD-L1阳性)的肿瘤的检测。
在本发明的第五方面,提供了一种本发明第一方面所述的免疫偶联物的用途,用于制备(a)体内检测PD-L1分子的检测试剂、检测试剂盒或检测板;(b)治疗或预防表达PD-L1蛋白(即PD-L1阳性)的肿瘤的药物组合物。
在本发明的另一方面,提供了一种本发明第一方面所述的免疫偶联物的用途,用于制备体内检测PD-L1分子的造影剂。
在本发明的第六方面,提供了一种抗PD-L1纳米抗体的VHH链,所述VHH链的氨基酸序列如SEQ ID NO.:1-7中任一所示。
在另一优选例中,所述的PD-L1为人PD-L1。
此外,还提供一种抗PD-L1纳米抗体的VHH链,所述的VHH包括框架区FR和互补决定区CDR,其中,所述的CDR包括SEQ ID NO.:1-7中任一序列中相应的CDR1、CDR2 和CDR3,以及被所述CDR1-3所隔开的FR1、FR2、FR3和FR4。
此外,还提供一种抗人PD-L1抗体的重链可变区,所述的重链可变区包括三个互补决定区CDR1、CDR2、和CDR3,并且3个CDR包括SEQ ID NO.:1-7中任一序列中相应的CDR1、CDR2和CDR3。
在本发明的第七方面,提供了一种抗PD-L1纳米抗体,它是针对PD-L1表位的纳米抗体,并且具有如SEQ ID NO.:1-7中任一所示的氨基酸序列的VHH链。
在本发明的第八方面,提供了一种多核苷酸,所述多核苷酸编码选自下组的蛋白质:第六方面所述的抗PD-L1纳米抗体的VHH链,或第七方面所述的抗PD-L1纳米抗体。
在另一优选例中,所述的多核苷酸包括DNA或RNA。
在另一优选例中,所述的多核苷酸具有如SEQ ID NO.:151-300中任一所示的核苷酸序列。
在本发明的第九方面,提供了一种表达载体,所述表达载体含有第八方面所述的多核苷酸。
在本发明的第十方面,提供了一种宿主细胞,所述宿主细胞含有第九方面所述的表达载体,或其基因组中整合有第八方面所述的多核苷酸。
在另一优选例中,所述的宿主细胞包括原核细胞或真核细胞。
在另一优选例中,所述的宿主细胞选自下组:大肠杆菌、酵母细胞。
在本发明的第十一方面,提供了一种产生抗PD-L1纳米抗体的方法,包括步骤:
(a)在适合产生纳米抗体的条件下,培养第十方面所述的宿主细胞,从而获得含所述抗PD-L1纳米抗体的培养物;以及
(b)从所述培养物中分离或回收所述的抗PD-L1纳米抗体。
在另一优选例中,所述的抗PD-L1纳米抗体具有如SEQ ID NO.:1-7中任一所示的氨基酸序列。
在本发明的第十二方面,提供了一种治疗疾病的方法,所述方法包括,给需要的对象施用本发明的纳米抗体或免疫偶联物。
在另一优选例中,所述的对象包括哺乳动物,如人。
应理解,在本发明范围内中,本发明的上述各技术特征和在下文(如实施例)中具体描述的各技术特征之间都可以互相组合,从而构成新的或优选的技术方案。限于篇幅,在此不再一一累述。
附图说明
图1显示了抗PD-L1纳米抗体纯化图。泳道M为分子量标准品,泳道1-7分别对应氨基酸序列如SEQ ID NO.:1-7所示的纳米抗体。
图2显示了抗PD-L1纳米抗体ELISA结果棒型图。棒型1-7分别对应氨基酸序列如SEQ ID NO.:1-7所示的纳米抗体。
图3显示了抗PD-L1纳米抗体HPLC谱图。分别对应抗PD-L1纳米抗体与小鼠或人血清共同孵育不同时间后的含量和组分测定,显示了抗PD-L1纳米抗体的稳定性。
图4显示了I-125标记抗PD-L1纳米抗体在PD-L1高表达荷瘤鼠SPECT图像。从左到右分别对应氨基酸序列如SEQ ID NO.:1-7所示的纳米抗体。
图5显示了本发明纳米抗体的氨基酸序列比对结果。
注:附图中的SEQ NO.与SEQ ID NO.具有相同含义,均表示序列表中的序列编号。
具体实施方式
本发明人经过广泛而深入地研究,首次意外地发现一种用于检测PD-L1分子的免疫偶联物,所述的免疫偶联物包含特定的抗PD-L1纳米抗体的VHH链和放射性核素,可以用于待测对象PD-L1表达情况的非侵入性检测。本发明的免疫偶联物具有小尺寸和高度特异性,适合同时靶向原发及转移肿瘤的全身检测,准确度高,辐射剂量小。在此基础上完成本发明。
术语
如本文所用,术语“本发明纳米抗体”、“本发明的抗PD-L1纳米抗体”、“本发明PD-L1纳米抗体”可互换使用,均指特异性识别和结合于PD-L1(包括人PD-L1)的纳米抗体。特别优选的是VHH链的氨基酸序列如SEQ ID NO.:1-7中任一所示的纳米抗体。
本发明的各VHH链的氨基酸序列如下所示,其中,下划线区域表示CDR区。
SEQ ID NO.1:
QVQLQESGGGSVQTGGSLRLSCAASTSIYSNNYMAWFSQAPGKGREGVAAVYIDDGRPYYADS VKGRFTISLDSAKNTVYLQMNRLKPEDTAMYYCAAAPGPLSHNYWYTSANYDYWGQGTQVTVSS
SEQ ID NO.2:
QVQLQESGGGSVQTGGSLRLSCTASTSIYSNNYMAWFSQSPGKGREGVAAVYMDDGRPYYADS VKGRFTISLDSAKNTMYLQMNSLKPEDTAMYYCAAAPGPLSRNYWYTSANYDYWGQGTQVTVSS
SEQ ID NO.3:
QVQLQESGGGSVQAGGSLRLSCAASGYTYSSDGMGWFRQTPGKEREGVAAISPTGRRTEYADS VKGRFTISRDNNKNMLSLQMNSLKPEDTGMYYCAREGSWSFSLANSAVRSWGQGTQVTVSS
SEQ ID NO.4:
QVQLQESGGGSVQAGGSLRLSCAASGYTRSSHCMVWFRQAPGKEREGVALIYTGSGSTYYADS VKGRFTISQDNAKKTLYLQMNSLKPEDTAMYYCAAGTSSSSCPGLLGPPRYYNWGQGTQVTVSS
SEQ ID NO.5:
QVQLQESGGGLVQPGGSLRLSCAASGFTFSIKAMSWVRQAPGKGLEWVSTIDSGGGRRYYADS VKGRFTISRDNAKNTLYLQLSSLKTEDTAMYFCARCSDIYCYNGASYRGQGTQVTVSS
SEQ ID NO.6:
QVQLQESGGGLVQPGGSLRLSCIASGFTFSIMAMSWVRQAPGKGLEWVSTINSDGGKTYYADS VKGRFTISRDNAKNTLYLQLNSLRTEDMAMYYCRRCADIYCSGSGGWTGQGTQVTVSS
SEQ ID NO.7:
QVQLQESGGGLVQPGGSLRLSCAASGFTFSIRAMSWVRQAPGKGLEWVSTINSGGDSRYYADS VKGRFTISRDNAKNTMYLQLNSLKTEDTAMYYCVRCSDIYCYNGASYRGQGTQVTVSS
对本发明纳米抗体的氨基酸进行序列比对,结果如图5所示,本发明的纳米抗体可按CDR1,CDR2及CDR3氨基酸序列相似度细分为三组,同组纳米抗体差异主要在CDR3。
如本文所用,术语“抗体”或“免疫球蛋白”是有相同结构特征的约150000 道尔顿的异四聚糖蛋白,其由两个相同的轻链(L)和两个相同的重链(H)组成。每条轻链通过一个共价二硫键与重链相连,而不同免疫球蛋白同种型的重链间的二硫键数目不同。每条重链和轻链也有规则间隔的链内二硫键。每条重链的一端有可变区(VH),其后是多个恒定区。每条轻链的一端有可变区(VL),另一端有恒定区;轻链的恒定区与重链的第一个恒定区相对,轻链的可变区与重链的可变区相对。特殊的氨基酸残基在轻链和重链的可变区之间形成界面。
如本文所用,术语“单域抗体(VHH)”、“纳米抗体”(nanobody)具有相同的含义,指克隆抗体重链的可变区,构建仅由一个重链可变区组成的单域抗体(VHH),它是具有完整功能的最小的抗原结合片段。通常先获得天然缺失轻链和重链恒定区1(CH1)的抗体后,再克隆抗体重链的可变区,构建仅由一个重链可变区组成的单域抗体(VHH)。
如本文所用,术语“可变”表示抗体中可变区的某些部分在序列上有所不同,它形成了各种特定抗体对其特定抗原的结合和特异性。然而,可变性并不均匀地分布在整个抗体可变区中。它集中于轻链和重链可变区中称为互补决定区(CDR)或超变区中的三个片段中。可变区中较保守的部分称为构架区(FR)。天然重链和轻链的可变区中各自包含四个FR区,它们大致上呈β-折叠构型,由形成连接环的三个CDR相连,在某些情况下可形成部分β折叠结构。每条链中的 CDR通过FR区紧密地靠在一起并与另一链的CDR一起形成了抗体的抗原结合部位(参见Kabat等,NIH Publ.No.91-3242,卷I,647-669页(1991))。恒定区不直接参与抗体与抗原的结合,但是它们表现出不同的效应功能,例如参与抗体的依赖于抗体的细胞毒性。
如本领域技术人员所知,免疫偶联物及融合表达产物包括:药物、毒素、细胞因子(cytokine)、放射性核素、酶和其他诊断或治疗分子与本发明的抗体或其片段结合而形成的偶联物。本发明还包括与所述的抗PD-L1蛋白抗体或其片段结合的细胞表面标记物或抗原。
如本文所用,术语“重链可变区”与“VH”可互换使用。
如本文所用,术语“可变区”与“互补决定区(complementarity determiningregion,CDR)”可互换使用。
在本发明的一个优选的实施方式中,所述抗体的重链可变区包括三个互补决定区CDR1、CDR2、和CDR3。
在本发明的一个优选的实施方式中,所述抗体的重链包括上述重链可变区和重链恒定区。
在本发明中,术语“本发明抗体”、“本发明蛋白”、或“本发明多肽”可互换使用,都指特异性结合PD-L1蛋白的多肽,例如具有重链可变区的蛋白或多肽。它们可含有或不含起始甲硫氨酸。
本发明还提供了具有本发明抗体的其他蛋白质或融合表达产物。具体地,本发明包括具有含可变区的重链的任何蛋白质或蛋白质偶联物及融合表达产物(即免疫偶联物及融合表达产物),只要该可变区与本发明抗体的重链可变区相同或至少90%同源性,较佳地至少95%同源性。
一般,抗体的抗原结合特性可由位于重链可变区的3个特定的区域来描述,称为可变区域(CDR),将该段间隔成4个框架区域(FR),4个FR的氨基酸序列相对比较保守,不直接参与结合反应。这些CDR形成环状结构,通过其间的FR形成的β折叠在空间结构上相互靠近,重链上的CDR和相应轻链上的CDR构成了抗体的抗原结合位点。可以通过比较同类型的抗体的氨基酸序列来确定是哪些氨基酸构成了FR或CDR区域。
本发明抗体的重链的可变区特别令人感兴趣,因为它们中至少部分涉及结合抗原。因此,本发明包括那些具有带CDR的抗体重链可变区的分子,只要其 CDR与此处鉴定的CDR具有90%以上(较佳地95%以上,最佳地98%以上)的同源性。
本发明不仅包括完整的抗体,还包括具有免疫活性的抗体的片段或抗体与其他序列形成的融合蛋白。因此,本发明还包括所述抗体的片段、衍生物和类似物。
如本文所用,术语“片段”、“衍生物”和“类似物”是指基本上保持本发明抗体相同的生物学功能或活性的多肽。本发明的多肽片段、衍生物或类似物可以是(i)有一个或多个保守或非保守性氨基酸残基(优选保守性氨基酸残基)被取代的多肽,而这样的取代的氨基酸残基可以是也可以不是由遗传密码编码的,或(ii)在一个或多个氨基酸残基中具有取代基团的多肽,或(i ii)成熟多肽与另一个化合物(比如延长多肽半衰期的化合物,例如聚乙二醇)融合所形成的多肽,或(iv)附加的氨基酸序列融合到此多肽序列而形成的多肽(如前导序列或分泌序列或用来纯化此多肽的序列或蛋白原序列,或与6His标签形成的融合蛋白)。根据本文的教导,这些片段、衍生物和类似物属于本领域熟练技术人员公知的范围。
本发明抗体指具有PD-L1蛋白结合活性的、包括上述CDR区的多肽。该术语还包括具有与本发明抗体相同功能的、包含上述CDR区的多肽的变异形式。这些变异形式包括(但并不限于):一个或多个(通常为1-50个,较佳地1-30个,更佳地1-20个,最佳地1-10个)氨基酸的缺失、插入和/或取代,以及在C末端和/或N末端添加一个或数个(通常为20个以内,较佳地为10个以内,更佳地为5 个以内)氨基酸。例如,在本领域中,用性能相近或相似的氨基酸进行取代时,通常不会改变蛋白质的功能。又比如,在C末端和/或N末端添加一个或数个氨基酸通常也不会改变蛋白质的功能。该术语还包括本发明抗体的活性片段和活性衍生物。
该多肽的变异形式包括:同源序列、保守性变异体、等位变异体、天然突变体、诱导突变体、在高或低的严紧度条件下能与本发明抗体的编码DNA杂交的DNA所编码的蛋白、以及利用抗本发明抗体的抗血清获得的多肽或蛋白。
本发明还提供了其他多肽,如包含纳米抗体或其片段的融合蛋白。除了几乎全长的多肽外,本发明还包括了本发明纳米抗体的片段。通常,该片段具有本发明抗体的至少约50个连续氨基酸,较佳地至少约50个连续氨基酸,更佳地至少约80个连续氨基酸,最佳地至少约100个连续氨基酸。
在本发明中,“本发明抗体的保守性变异体”指与本发明抗体的氨基酸序列相比,有至多10个,较佳地至多8个,更佳地至多5个,最佳地至多3个氨基酸被性质相似或相近的氨基酸所替换而形成多肽。这些保守性变异多肽最好根据表1进行氨基酸替换而产生。
表1
最初的残基 | 代表性的取代 | 优选的取代 |
Ala(A) | Val;Leu;Ile | Val |
Arg(R) | Lys;Gln;Asn | Lys |
Asn(N) | Gln;His;Lys;Arg | Gln |
Asp(D) | Glu | Glu |
Cys(C) | Ser | Ser |
Gln(Q) | Asn | Asn |
Glu(E) | Asp | Asp |
Gly(G) | Pro;Ala | Ala |
His(H) | Asn;Gln;Lys;Arg | Arg |
Ile(I) | Leu;Val;Met;Ala;Phe | Leu |
Leu(L) | Ile;Val;Met;Ala;Phe | Ile |
Lys(K) | Arg;Gln;Asn | Arg |
Met(M) | Leu;Phe;Ile | Leu |
Phe(F) | Leu;Val;Ile;Ala;Tyr | Leu |
Pro(P) | Ala | Ala |
Ser(S) | Thr | Thr |
Thr(T) | Ser | Ser |
Trp(W) | Tyr;Phe | Tyr |
Tyr(Y) | Trp;Phe;Thr;Ser | Phe |
Val(V) | Ile;Leu;Met;Phe;Ala | Leu |
本发明还提供了编码上述抗体或其片段或其融合蛋白的多核苷酸分子。本发明的多核苷酸可以是DNA形式或RNA形式。DNA形式包括cDNA、基因组DNA或人工合成的DNA。DNA可以是单链的或是双链的。DNA可以是编码链或非编码链。
编码本发明的成熟多肽的多核苷酸包括:只编码成熟多肽的编码序列;成熟多肽的编码序列和各种附加编码序列;成熟多肽的编码序列(和任选的附加编码序列)以及非编码序列。
术语“编码多肽的多核苷酸”可以是包括编码此多肽的多核苷酸,也可以是还包括附加编码和/或非编码序列的多核苷酸。
本发明还涉及与上述的序列杂交且两个序列之间具有至少50%,较佳地至少70%,更佳地至少80%相同性的多核苷酸。本发明特别涉及在严格条件下与本发明所述多核苷酸可杂交的多核苷酸。在本发明中,“严格条件”是指:(1) 在较低离子强度和较高温度下的杂交和洗脱,如0.2×SSC,0.1%SDS,60℃;或(2)杂交时加有变性剂,如50%(v/v)甲酰胺,0.1%小牛血清/0.1%Ficoll, 42℃等;或(3)仅在两条序列之间的相同性至少在90%以上,更好是95%以上时才发生杂交。并且,可杂交的多核苷酸编码的多肽与成熟多肽有相同的生物学功能和活性。
本发明的抗体的核苷酸全长序列或其片段通常可以用PCR扩增法、重组法或人工合成的方法获得。一种可行的方法是用人工合成的方法来合成有关序列,尤其是片段长度较短时。通常,通过先合成多个小片段,然后再进行连接可获得序列很长的片段。此外,还可将重链的编码序列和表达标签(如6His)融合在一起,形成融合蛋白。
一旦获得了有关的序列,就可以用重组法来大批量地获得有关序列。这通常是将其克隆入载体,再转入细胞,然后通过常规方法从增殖后的宿主细胞中分离得到有关序列。本发明所涉及的生物分子(核酸、蛋白等)包括以分离的形式存在的生物分子。
目前,已经可以完全通过化学合成来得到编码本发明蛋白(或其片段,或其衍生物)的DNA序列。然后可将该DNA序列引入本领域中已知的各种现有的DNA 分子(或如载体)和细胞中。此外,还可通过化学合成将突变引入本发明蛋白序列中。
本发明还涉及包含上述的适当DNA序列以及适当启动子或者控制序列的载体。这些载体可以用于转化适当的宿主细胞,以使其能够表达蛋白质。
宿主细胞可以是原核细胞,如细菌细胞;或是低等真核细胞,如酵母细胞;或是高等真核细胞,如哺乳动物细胞。代表性例子有:大肠杆菌,链霉菌属;鼠伤寒沙门氏菌的细菌细胞;真菌细胞如酵母;果蝇S2或Sf9的昆虫细胞;CHO、COS7、293细胞的动物细胞等。
用重组DNA转化宿主细胞可用本领域技术人员熟知的常规技术进行。当宿主为原核生物如大肠杆菌时,能吸收DNA的感受态细胞可在指数生长期后收获,用CaCl2法处理,所用的步骤在本领域众所周知。另一种方法是使用MgCl2。如果需要,转化也可用电穿孔的方法进行。当宿主是真核生物,可选用如下的DNA 转染方法:磷酸钙共沉淀法,常规机械方法如显微注射、电穿孔,脂质体包装等。
获得的转化子可以用常规方法培养,表达本发明的基因所编码的多肽。根据所用的宿主细胞,培养中所用的培养基可选自各种常规培养基。在适于宿主细胞生长的条件下进行培养。当宿主细胞生长到适当的细胞密度后,用合适的方法(如温度转换或化学诱导)诱导选择的启动子,将细胞再培养一段时间。
在上面的方法中的重组多肽可在细胞内、或在细胞膜上表达、或分泌到细胞外。如果需要,可利用其物理的、化学的和其它特性通过各种分离方法分离和纯化重组的蛋白。这些方法是本领域技术人员所熟知的。这些方法的例子包括但并不限于:常规的复性处理、用蛋白沉淀剂处理(盐析方法)、离心、渗透破菌、超处理、超离心、分子筛层析(凝胶过滤)、吸附层析、离子交换层析、高效液相层析(HPLC)和其它各种液相层析技术及这些方法的结合。
本发明的抗体可以单独使用,也可与可检测标记物(为诊断目的)、治疗剂、 PK(蛋白激酶)修饰部分或任何以上这些物质的组合结合或偶联。
用于诊断目的可检测标记物包括但不限于:荧光或发光标记物、放射性标记物、MRI(磁共振成像)或CT(电子计算机X射线断层扫描技术)造影剂、或能够产生可检测产物的酶。优选的可检测标记物为放射性核素。
可与本发明抗体结合或偶联的治疗剂包括但不限于:1.放射性核素;2. 生物毒;3.细胞因子如IL-2等;4.金纳米颗粒/纳米棒;5.病毒颗粒;6.脂质体;7.纳米磁粒;8.前药激活酶(例如,DT-心肌黄酶(DTD)或联苯基水解酶 -样蛋白质(BPHL));10.化疗剂(例如,顺铂)或任何形式的纳米颗粒等。
免疫偶联物
本发明还提供了一种免疫偶联物,所述的免疫偶联物含有:
(a)抗PD-L1纳米抗体的VHH链或具有所述的VHH链的抗PD-L1纳米抗体,其中,所述的VHH链的氨基酸序列如SEQ ID NO.:1-7中任一所示;和
(b)选自下组的偶联部分:放射性核素、酶抗体、细胞、或其组合。
在另一优选例中,所述偶联部分为放射性核素。
在另一优选例中,所述偶联部分为药物或毒素。
在另一优选例中,所述偶联部分为可检测标记物。
在另一优选例中,所述偶联物选自:荧光或发光标记物、放射性标记物、MRI(磁共振成像)或CT(电子计算机X射线断层扫描技术)造影剂、或能够产生可检测产物的酶、放射性核素、生物毒素、细胞因子(如IL-2等)、抗体、抗体Fc片段、抗体 scFv片段、金纳米颗粒/纳米棒、病毒颗粒、脂质体、纳米磁粒、前药激活酶(例如,DT-心肌黄酶(DTD)或联苯基水解酶-样蛋白质(BPHL))、化疗剂(例如,顺铂) 或任何形式的纳米颗粒等。
本发明的免疫偶联物可以用于非侵入性地检测待测对象的PD-L1表达,具有小尺寸和高度特异性,适合同时靶向原发及转移肿瘤的全身检测,准确度高,辐射剂量小。
试剂盒
本发明还提供了一种含有本发明的免疫偶联物的试剂盒,在本发明的一个优选例中,所述的试剂盒还包括容器、使用说明书、同位素示踪剂以及选自下组的一种或多种试剂:造影剂、流式检测试剂、细胞免疫荧光检测试剂、纳米磁粒和显像剂。
优选的,本发明的试剂盒是体内诊断试剂盒,用于非侵入性地检测待测对象的PD-L1表达。
细胞毒剂
构成本发明抗体偶联物的偶联部分包括:毒素,如细菌、真菌、植物或动物来源的小分子毒素或酶活性毒素,包括其片段和/或变体。细胞毒剂的例子包括但不限于:耳他汀类(例如,耳他汀E、耳他汀F、MMAE和MMAF)、金霉素、类美坦西醇、篦麻毒素、篦麻毒素A-链、考布他汀、多卡米星、多拉司他汀、阿霉素、柔红霉素、紫杉醇、顺铂、cc1065、溴化乙锭、丝裂霉素、依托泊甙、替诺泊甙(tenoposide)、长春新碱、长春碱、秋水仙素、二羟基炭疽菌素二酮、放线菌素、白喉毒素、假单胞菌外毒素(PE)A、PE40、相思豆毒素、相思豆毒素A链、蒴莲根毒素A链、α-八叠球菌、白树毒素、迈托毒素(mitogellin)、局限曲菌素(retstrictocin)、酚霉素、依诺霉素、麻疯树毒蛋白(curicin)、巴豆毒素、卡奇霉素、肥皂草(Sapaonariaofficinalis)抑制剂以及糖皮质激素和其它化学治疗剂,以及放射性同位素,如 At211、I131、I125、Y90、Re186、Re188、Sm153、Bi212或213、P32和包括Lu177在内的Lu的放射性同位素。抗体也可与能够将前药转化成其活性形式的抗癌前药活化酶偶联。
优选的小分子药物为具有高细胞毒性的化合物,优选单甲基澳瑞他汀(monomethylauristatin)、加利车霉素、美登素类、或其组合;更佳地选自:单甲基澳瑞他汀-E(MMAE)、单甲基澳瑞他汀-D(MMAD)、单甲基澳瑞他汀-F(MMAF)、或其组合。
药物组合物
本发明还提供了一种组合物。优选地,所述的组合物是药物组合物,它含有上述的抗体或其活性片段或其融合蛋白,以及药学上可接受的载体。通常,可将这些物质配制于无毒的、惰性的和药学上可接受的水性载体介质中,其中 pH通常约为5-8,较佳地pH约为6-8,尽管pH值可随被配制物质的性质以及待治疗的病症而有所变化。配制好的药物组合物可以通过常规途径进行给药,其中包括(但并不限于):瘤内、腹膜内、静脉内、或局部给药。
本发明的药物组合物可直接用于结合PD-L1蛋白分子,因而可用于治疗肿瘤。此外,还可同时使用其他治疗剂。
本发明的药物组合物含有安全有效量(如0.001-99wt%,较佳地 0.01-90wt%,更佳地0.1-80wt%)的本发明上述的纳米抗体(或其偶联物)以及药学上可接受的载体或赋形剂。这类载体包括(但并不限于):盐水、缓冲液、葡萄糖、水、甘油、乙醇、及其组合。药物制剂应与给药方式相匹配。本发明的药物组合物可以被制成针剂形式,例如用生理盐水或含有葡萄糖和其他辅剂的水溶液通过常规方法进行制备。药物组合物如针剂、溶液宜在无菌条件下制造。活性成分的给药量是治疗有效量,例如每天约10微克/千克体重-约50毫克/千克体重。此外,本发明的多肽还可与其他治疗剂一起使用。
使用药物组合物时,是将安全有效量的免疫偶联物施用于哺乳动物,其中该安全有效量通常至少约10微克/千克体重,而且在大多数情况下不超过约50 毫克/千克体重,较佳地该剂量是约10微克/千克体重-约10毫克/千克体重。当然,具体剂量还应考虑给药途径、病人健康状况等因素,这些都是熟练医师技能范围之内的。
本发明的主要优点包括:
(a)本发明的免疫偶联物同时靶向原发及转移肿瘤,全身显像,一次定位、定性、定量、分期。
(b)本发明的免疫偶联物具有小尺寸及高度特异性的特点,能够更有效渗透肿瘤组织及更容易被身体排走,从而降低对非靶向组织的放辐射剂量。
(c)本发明的免疫偶联物具有短半衰期及更短的诊断时间,快速观察结果。
(d)本发明的免疫偶联物具有高度特异性,检测准确,避免局部假阴性。
下面结合具体实施例,进一步阐述本发明。应理解,这些实施例仅用于说明本发明而不用于限制本发明的范围。下列实施例中未注明具体条件的实验方法,通常按照常规条件,或按照制造厂商所建议的条件。除非另外说明,否则百分比和份数按重量计算。
实施例1纳米抗体在宿主菌大肠杆菌中表达、纯化
(1)将纳米抗体(序列如SEQ ID NO.:1-7所示)的相应质粒电转化到大肠杆菌WK6中,并将其涂布在LA+glucose即含有氨苄青霉素和葡萄糖的培养平板上, 37℃培养过夜。
(2)挑选单个菌落接种在5mL含有氨苄青霉素的LB培养液中,37℃摇床培养过夜。
(3)接种1mL的过夜菌种至330mL TB培养液中,37℃摇床培养,培养到 OD值达到0.6-1时,加入IPTG,28℃摇床培养过夜。
(4)离心收菌,利用渗透法获得抗体粗提液。
(5)利用渗透法,获得抗体粗提液。
(6)经镍柱离子亲和层析制备纯度达90%以上的纳米抗体。
纯化结果如图1所示,制备的纳米抗体的纯度均达95%以上。
实施例2酶联免疫法(ELISA)鉴定纳米抗体的亲和力
(1)包被抗原蛋白PD-L1及IgG:每孔0.5μg(5μg/mL,100μL),包被 NaHCO3(100mM,Ph8.2)为空白对照,4℃过夜。
(2)第二天用PBST洗涤3次,加入200μL的1%BSA室温下封闭2小时。
(3)将每株纯化的纳米抗体稀释至10μg/mL,分别取100μL与包被的 PD-L1、PD-L2及空白对照组孵育,室温下反应1小时。
(4)用PBST洗去未结合的抗体,加入100μL mouse anti-HA tag antibody(1:2000稀释),在室温下放置1小时。
(5)用PBST洗去未结合的抗体,加入anti-mouse alkaline phosphataseconjugate(1:2000稀释),在室温下放置1小时。
(6)用PBST洗去未结合的抗体,加入碱性磷酸酶显色液,于ELISA仪上,在 405nm波长,读取吸收值。根据吸收值判断纳米抗体的特异性。
检测结果如图2所示,本发明的纳米抗体对PD-L1具有极好的亲和力。
通过梯度稀释纳米抗体对其亲和力进行进一步测定。
结果如表2所示,结果显示本发明的纳米抗体亲和力达到1x10-9以上。
表2抗PD-L1纳米抗体的亲和力和特异性
实施例3流式细胞术检测纳米抗体是否具有阻断PD-1与PD-L1结合的作用
(1)取1×106个瞬转表达人PD-L1全长蛋白的HEK293F细胞重悬于0.5% BSA-PBSbuffer中,加入抗PD-L1纳米抗体10μg,同时设置阳性对照,阴性对照和空白组(PBS),所有样本加入5μg hPD-1-Fc-Biotin,4℃孵育20min。
(2)PBS洗涤2次细胞,加入eBioscience的SA-PE,4℃孵育20min,PBS洗涤 2次细胞后用流式细胞仪检测。
结果如表2 所示,结果显示本发明的纳米抗体不能阻断PD-1与PD-L1结合的作用。
实施例4流式细胞术检测纳米抗体的特异性
(1)每个样品取2×105天然表达PD-L1蛋白(HCC827、A549)的细胞系细胞并重悬于0.5%BSA-PBS buffer中,分别加入九种10μg纯化的抗PD-L1纳米抗体,同时设置阳性对照、阴性对照和空白组(PBS),4℃孵育20min。
(2)PBS洗涤2次细胞,加入anti-humanIgG-FITC,4℃孵育20min,PBS洗涤 2次细胞后上机检测(BD FACS Calibur)。
结果如表2所示,在PD-L1高表达(HCC827)的细胞株,纳米抗体的阳性率为 67-94%,在PD-L1低表达(A549)的细胞株,纳米抗体的阳性率为14-45%,两者相差至少约2倍,这进一步提示本发明纳米抗体具有非常优异针对PD-L1的特异性。
实施例5纳米抗体99mTc标记,分离纯化及血清稳定性试验
(1)分别加入Na2CO3 5.5mg、酒石酸钾钠15.2mg和NaBH4 20.5mg至10mL无菌瓶,通入20min CO,再加入1mL(35mCi)Na[99mTcO4],密封反应瓶,于80 ℃下加热30min。
(2)取抗体原液溶液50μl,加入500μl 99mTc(CO)3(H2O)3反应液 (6.56mCi),于45-50℃下反应90min。
(3)用PD10柱分离,洗脱液为0.02mol/L pH7.4磷酸缓冲溶液,用薄层色谱法对99mTc标记纳米抗体进行放射纯度鉴定。
(4)取100μl 99mTc标记纳米抗体,加入500μl老鼠或人血清,37℃孵育 30,90及180min。
(5)用分子排阻HPLC对孵育99mTc标记纳米抗体进行分析。
结果见图3所示,HPLC谱图显示本发明的纳米抗体在血清体外孵育180min 亦没有任何降解,十分稳定。
实施例6纳米抗体I-125标记,分离纯化及SPECT显像扫描
(1)取抗体原液150μL,加入100μL 0.02mol/L pH7.4磷酸盐缓冲溶液和 50μLNa125I溶液,混匀,加入20μL 5mg/mL氯胺T溶液,混匀器上室温下反应70s,加入200μL偏重亚硫酸钠溶液(5mg/mL)作用5分钟。
(2)用PD10柱分离,洗脱液为0.02mol/L pH7.4磷酸缓冲溶液,每管收集10 滴,用纸层析对I-125标记纳米抗体进行放射纯度鉴定。
(3)在裸鼠右侧腋下接种5×105个PD-L1高表达(HCC827)细胞,待肿瘤长至 150-200mm3用于正式实验研究。
(4)通过异氟烷麻醉荷瘤鼠,尾静脉注射I-125标记纳米抗体(~50ug, 5MBq)
(5)给药后0.5hr进行扫描,采集方式为静态15min SPECT、中分辨率全身CT。
图4和表3显示了荷瘤鼠30min SPECT扫描图片及身体内分布数据,结果显示本发明的纳米抗体能够有效于PD-L1高表达肿瘤模型有效积聚,可非侵入性检测PD-L1表达,应用于癌症预后及诊断。同时非结合抗体能够快速透过肾脏和膀胱从血液清除,减低身体放射性剂量,同时缩短等待数描时间。
表3 I-125标记抗PD-L1纳米抗体在PD-L1高表达荷瘤鼠的体内分布
在本发明提及的所有文献都在本申请中引用作为参考,就如同每一篇文献被单独引用作为参考那样。此外应理解,在阅读了本发明的上述讲授内容之后,本领域技术人员可以对本发明作各种改动或修改,这些等价形式同样落于本申请所附权利要求书所限定的范围。
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<110> 苏州纳洛迈生物科技有限公司
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Claims (16)
1.一种免疫偶联物,其特征在于,所述的免疫偶联物含有:
(a)抗PD-L1纳米抗体的重链可变区或具有所述的重链可变区的抗PD-L1纳米抗体,其中,所述的重链可变区的氨基酸序列如SEQ ID NO.3所示;和
(b)选自下组的偶联部分:细胞毒性药物、毒素、或放射性核素,其中,所述的放射性核素包括:
(i)诊断用同位素,所述的诊断用同位素选自下组:Tc-99m、Ga-68、F-18、I-123、I-125、In-111、Ga-67、Cu-64、Zr-89、C-11、或其组合;或
(ii)治疗用同位素,所述的治疗用同位素选自下组:Lu-177、Y-90、Ac-225、As-211、Bi-212、Bi-213、Cs-137、Cr-51、Co-60、Dy-165、Er-169、Fm-255、Au-198、Ho-166、I-125、I-131、Ir-192、Fe-59、Pb-212、Mo-99、Pd-103、P-32、K-42、Re-186、Re-188、Sm-153、Ra223、Ru-106、Na24、Sr89、Tb-149、Th-227、Xe-133Yb-169、Yb-177或其组合,
并且,所述的毒素选自下组:
篦麻毒素、篦麻毒素A-链、溴化乙锭、秋水仙素、二羟基炭疽菌素二酮、白喉毒素、假单胞菌外毒素A、相思豆毒素、相思豆毒素A链、蒴莲根毒素A链、α-八叠球菌、迈托毒素(mitogellin)、局限曲菌素、麻疯树毒蛋白、巴豆毒素、或其组合。
2.如权利要求1所述的免疫偶联物,其特征在于,所述的放射性核素选自下组:Tc-99m、I-125、或其组合。
3.如权利要求1所述的免疫偶联物,其特征在于,所述的细胞毒性药物选自下组:
抗微管蛋白药物、DNA小沟结合试剂、DNA复制抑制剂、抗代谢药物、拓扑异构酶抑制剂。
4.如权利要求1所述的免疫偶联物,其特征在于,所述的细胞毒性药物选自下组:
烷化试剂、抗生素、叶酸拮抗物、长春花生物碱。
5.如权利要求1所述的免疫偶联物,其特征在于,所述的偶联部分选自下组:
耳他汀类、金霉素、阿霉素、柔红霉素、cc1065、丝裂霉素、放线菌素、酚霉素、依诺霉素、卡奇霉素、考布他汀、多拉司他汀、紫杉醇、长春新碱、长春碱、依托泊甙、替诺泊甙(tenoposide)。
6.如权利要求5所述的免疫偶联物,其特征在于,所述的耳他汀类选自下组:耳他汀E、耳他汀F、MMAE、MMAF、或其组合。
7.如权利要求1所述的免疫偶联物,其特征在于,所述的免疫偶联物含有多价的所述重链可变区。
8.一种PD-L1蛋白检测试剂,其特征在于,所述的检测试剂包含权利要求1所述的免疫偶联物和检测学上可接受的载体。
9.如权利要求8所述的检测试剂,其特征在于,所述的免疫偶联物的偶联部分为诊断用同位素。
10.如权利要求8所述的检测试剂,其特征在于,所述的检测试剂被用作选自下组的一种或多种试剂:同位素示踪剂、造影剂、流式检测试剂、细胞免疫荧光检测试剂、纳米磁粒和显像剂。
11.如权利要求10所述的检测试剂,其特征在于,所述的造影剂是用于磁共振成像或电子计算机X射线断层扫描技术的造影剂。
12.一种药物组合物,其特征在于,所述的药物组合物包含权利要求1所述的免疫偶联物和药学上可接受的载体。
13.如权利要求12所述的药物组合物,其特征在于,所述的免疫偶联物的偶联部分为细胞毒性药物和/或治疗用同位素。
14.一种检测PD-L1蛋白的试剂盒,其特征在于,所述试剂盒含有权利要求1所述的免疫偶联物和说明书。
15.权利要求1所述的免疫偶联物的用途,其特征在于,用于制备体内检测PD-L1分子的检测试剂、检测试剂盒或检测板。
16.权利要求1所述的免疫偶联物的用途,其特征在于,所述的免疫偶联物的偶联部分为细胞毒性药物、毒素或治疗用同位素,并且其用于制备治疗表达PD-L1蛋白的肿瘤的药物组合物。
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