CN101045156A - 特异靶向性药物及其用途 - Google Patents
特异靶向性药物及其用途 Download PDFInfo
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- CN101045156A CN101045156A CNA2006100251857A CN200610025185A CN101045156A CN 101045156 A CN101045156 A CN 101045156A CN A2006100251857 A CNA2006100251857 A CN A2006100251857A CN 200610025185 A CN200610025185 A CN 200610025185A CN 101045156 A CN101045156 A CN 101045156A
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Abstract
本发明公开了一种特异靶向性药物、编码该种特异靶向性药物的核酸序列、含有该核酸序列的表达载体以及由该载体转化的宿主细胞,本发明还公开了特异靶向性药物在制备治疗肝脏疾病的药物中的应用。本发明的特异靶向性药物将介导肝细胞特异性感染的病毒蛋白或多肽与治疗性药物相连接,产生的特异靶向性药物可对病毒性肝炎、肝硬化、肝脏肿瘤等肝脏疾病进行靶向治疗,在增强药物疗效的同时又降低药物对肝脏以外器官造成的不良反应。
Description
技术领域
本发明涉及特异靶向性药物,尤其涉及一种用于治疗病毒性肝炎、肝硬化、肝脏肿瘤等肝脏疾病的特异靶向性药物。
背景技术
病毒对宿主细胞的特异性选择在病毒感染的现象中广泛存在。自然界中存在一类对肝细胞具有特异或相对特异性感染的病毒,称之为嗜肝病毒。目前已被公认的人类嗜肝病毒有人甲、乙、丙、丁、戊型肝炎病毒,“庚型肝炎病毒”和新发现的输血传播病毒TTV(含其变异株SANBAN、YONBAN等)、SENV(TTV相关病毒)、TLMV(TTV样微小病毒)、CAV(鸡白血病病毒)可以引起肝炎病变,但目前尚未被公认为嗜肝病毒。另外,临床上约有10%的病毒性肝炎的病因目前尚未确定,称之为未分型肝炎病毒。与人乙型肝炎病毒同属嗜肝去氧核糖核酸病毒的还有土拨鼠肝炎病毒、地松鼠肝炎病毒和鸭肝炎病毒。
肝炎病毒的嗜肝特异性主要依赖病毒蛋白与肝细胞表面的病毒受体或辅受体特异性结合,从而实现嗜肝病毒对肝细胞的特异性感染。人甲型肝炎病毒(hepatitis Avirus,HAV)属小RNA病毒科嗜肝RNA病毒属。甲型肝炎病毒衣壳蛋白VP1上的细胞受体结合区与肝细胞表面的受体(HAV cellular receptor-1,HAVcr-1)结合,介导HAV对肝细胞的特异性感染(Kaplan,G.,A.Totsuka,P.Thompson,T.Akatsuka,Y.Moritsugu,and S.M.Feinstone.1996.Identification of a surface glycoproteinon African green monkey kidney cells as a receptor for hepatitis A virus.EMBOJ.15:4282-4296.;Feigelstock,D.,P.Thompson,P.Mattoo,Y.Zhang,and G.G.Kaplan.1998.The human homolog of HAVcr-1 codes for a hepatitis A viruscellular receptor.J.Virol.72:6621-6628.)。丙型肝炎病毒(hepatitis C virus,HCV)属于黄病毒科,核心为单股正链RNA,病毒包膜上存在E1、E2两种糖蛋白,其中E2被证实是介导HCV感染肝细胞的关键蛋白,其肝细胞表面的对应受体可能是CD81,HCV E2糖蛋白的第480-493及544-551位氨基酸是结合CD81的关键部位。人乙型肝炎病毒(hepatitis B virus,HBV)属嗜肝DNA病毒科,其病毒包膜上存在3种表面蛋白,分别称为大、中、小表面蛋白。其中HBV表面大蛋白Pre-S1区存在与肝细胞特异性受体或辅受体结合的关键氨基酸序列,并定位于Pre-S1的第2到第47位氨基酸,但相应的肝细胞膜表面受体目前尚未明确。人丁和戊型肝炎病毒及其他肝炎病毒的嗜肝特异性机理尚未明确。
利用嗜肝病毒的嗜肝特异性分子机制可介导肝局域性疾病的药物靶向治疗。肝局域性疾病包括病毒性肝炎、肝部肿瘤、肝硬化及其他肝局域性疾病。HBV感染是全球最严重的公共卫生问题之一,全球约有20亿人感染过HBV,慢性HBV感染者超过3.5亿。每年与HBV感染相关的死亡人数高达100万,每年新增感染估计是HIV新增感染的2.5~4倍。世界上75%的HBV慢性感染者集中在亚洲(约为2.87亿),中国是乙型肝炎的高流行区,70年代末和90年代初两次全国肝炎流行病学调查的数据显示,我国感染过HBV者6.9亿,感染率为57.6%,全国长期携带HBV者1.2亿,HBV表面抗原携带率9.75%,现有的慢性乙型肝炎患者2000余万。丙型病毒性肝炎也呈全球性分布,目前全世界有1.7亿人感染HCV,美国大约有HCV感染者390万,我国丙型肝炎病毒携带者3800万人,丙型病毒性肝炎占全球慢性肝炎的60%至70%,约有50%的晚期肝硬化和肝癌由该病毒引起,在美国是引起肝移植手术的主要病因。肝癌全世界每年新发病例26万,占恶性肿瘤的4%,分别位于男性和女性恶性肿瘤的第7和第9位。我国肝癌约占世界的42.5%,是我国第3位高发肿瘤,占各种肿瘤死亡的15%,其导致的人群死亡率高达20.1/10万人口。肝癌高度恶性,其5年生存率仅为5%。
目前用于治疗肝部疾病的药物包括抗肝癌药物、核苷类似物抗肝炎病毒药物和治疗肝部疾病的细胞因子,其中以干扰素(interferon,IFN)应用最多。IFN是一类相对小分子量单链蛋白,由Isaaca和Lindenmann于1957年首先发现,迄今为止已经鉴定的人干扰素有近30种,所知的人、鼠、牛、猪、马等哺乳动物的IFN基于生理化学和生物的差异均分为IFN-alpha(IFNα)、IFN-beta(IFNβ)、IFN-gamma(IFNγ)、IFN-omega(IFNω)、IFN-kappa(IFNκ)、IFN-tau(IFNτ)和IFN-Delta(IFNδ)。其中IFN-a型中又有许多亚型,如α-1a型、α-1b型、α-2a型及a-2b型,亚型成员有20种以上。人IFN-a由166或165个氨基酸组成,分子量在19000道尔顿左右。目前公认的IFN生物学功能包括广谱的抗病毒活性、抗肿瘤和免疫调节三大功能,其中以抗病毒活性最为公认,因而IFN被广泛应用于慢性乙型和丙型病毒性肝炎、肿瘤、白血病等多种疾病的治疗。IFN是被美国FDA批准上市种类最多、销售额最高的生物技术产品之一。目前全球HBV和HCV感染者分别高达3.5亿和1亿,中国乙型和丙型病毒性肝患者高达3000万人。虽然IFN-a是迄今为止治疗病毒性肝炎具有肯定疗效的药物,但是由于其血清中半衰期仅有数小时(参见Physician’s DeskReference),因此为了达到相当的药效就必须注射高剂量的IFN。这不仅使IFN的临床应用出现较大的不良副作用(包括神经、内分泌和免疫系统毒性),而且由于这些毒性限制了IFN给药剂量的进一步提高,导致临床疗效尚不理想。由于IFN治疗病毒性肝炎或肝脏肿瘤等肝区域性疾病时,仅有肝部IFN才发挥主要的治疗作用,而肝脏之外的IFN则是造成肝外不良反应的主要原因。因此仅通过聚乙二醇偶联、蛋白偶联等方式延长IFN体内半衰期(J.Pharmaceut.Sci.,83:601-606,1994),虽然能延长给药时间间隔、减少给药次数,但不能有效降低IFN引起的不良反应,也不能提高给药剂量而提高IFN的疗效。
发明内容
本发明要解决的技术问题之一是提供一种特异靶向性药物,该药物将介导肝细胞特异性感染的病毒蛋白或多肽与药物相结合,利用病毒蛋白或多肽介导药物靶向肝脏,从而治疗病毒性肝炎等肝脏局域性疾病。
本发明要解决的技术问题之二是提供一种编码特异靶向性药物的核酸分子。
本发明要解决的技术问题之三是提供一种包含上述编码特异靶向性药物核酸分子的载体。
本发明要解决的技术问题之四是提供一种包含上述载体的宿主细胞。
本发明要解决的技术问题之五是提供一种药物组合物,该组合物含有安全有效量的特异靶向性药物和药学上可接受的载体。
本发明要解决的技术问题之六是提供所述特异靶向性药物在制备治疗肝脏疾病的药物中的应用。
为了解决上述技术问题,本发明采用如下技术方案:
在本发明的一个方面,提供了一种特异靶向性药物,它具有通式X-L-Y,其中,
X表示氨基酸序列,该序列包含:(a)来源于具有肝脏特异性或相对特异性感染病毒的蛋白的氨基酸序列,(b)由(a)的序列发生一个或多个氨基酸残基的置换、缺失、插入或添加且与(a)具有相同活性的氨基酸序列,所述病毒蛋白与细胞感染受体或辅受体相结合,并介导或辅助病毒的感染;
L表示X与Y之间的任一连接,该连接可缺失;
Y表示对正常细胞、病理状态下细胞、受感染细胞、肿瘤细胞及病原微生物具有药理或生理作用的药物和或基团;
所述X和Y的位置可颠倒,X、L、Y之间可进行单一或多倍的排列组合,且多倍排列组合中的各X或Y可相同或不同。
较佳地,所述具有肝脏特异性或相对特异性感染病毒包括甲型肝炎病毒、乙型肝炎病毒、丙型肝炎病毒、丁型肝炎病毒、戊型肝炎病毒及未分型肝炎病毒;尤其较佳地,所述X序列包含:人乙型肝炎病毒表面大蛋白Pre-S1的多肽,或其保守性变异多肽、或其活性片段,或其活性衍生物;更佳地,所述X序列包含:具有SEQ ID NO:1氨基酸序列的人乙型肝炎病毒表面大蛋白Pre-S1多肽,或其保守性变异多肽、或其活性片段,或其活性衍生物;尤其更佳地,所述X序列选自下组:(a)具有SEQ ID NO:1氨基酸序列的多肽,(b)将SEQ ID NO:1氨基酸序列经过一个或几个氨基酸残基的置换、缺失、插入或添加且具有与SEQ ID NO:1氨基酸序列相同活性的由(a)衍生的多肽;特别优选X为具有SEQ ID NO:3氨基酸序列的多肽。
较佳地,所述Y是对正常肝细胞、病理状态下肝细胞、受感染肝细胞、肝肿瘤细胞及肝细胞内病毒或病原微生物具有药理或生理作用的药物,包括蛋白质、多肽、细胞毒性药物、小分子药物及放射性药物;尤其较佳地,所述Y为蛋白质药物,包括细胞因子、干扰素、白细胞介素、生长因子、集落刺激因子、趋化因子及该类蛋白质药物的突变体;更佳地,所述Y包含:干扰素α、干扰素β、干扰素γ、干扰素ω、干扰素κ、干扰素τ、干扰素δ,或其保守性变异蛋白质、或其活性片段,或其活性衍生物;尤其更佳地,所述Y选自下组:(a)具有SEQ ID NO:2氨基酸序列的干扰素α-2b,(b)由(a)的蛋白发生一个或多个氨基酸残基的置换、缺失、插入或添加且与(a)的干扰素α-2b具有相同活性的衍生蛋白质;特别优选Y为具有SEQ ID NO:5氨基酸序列的干扰素α-2b。
较佳地,所述L为X与Y之间的氨基酸连接;更佳地,所述L为主要由G(甘氨酸)、A(丙氨酸)、S(丝氨酸)和T(苏氨酸)四种氨基酸组成的氨基酸序列。
本发明的特异靶向性药物优选为具有SEQ ID NO:6的氨基酸序列,尤其优选SEQID NO:6氨基酸序列第15位氨基酸N(天冬酰氨)被氨基酸Q(谷氨酰氨)替换后产生的SEQ ID NO:7氨基酸序列,特别优选第13位氨基酸G(甘氨酸)被豆蔻酰化的SEQID NO:7氨基酸序列。
在本发明的另一方面,提供了一种核酸分子,它编码上述特异靶向性药物的氨基酸序列。
较佳地,所述核酸分子包括下列核苷酸序列之一:
(1)序列表中SEQ ID NO:8或SEQ ID NO:9的DNA序列;
(2)编码序列表中SEQ ID NO:7氨基酸序列的多核苷酸;
(3)与序列表中SEQ ID NO:8或SEQ ID NO:9的DNA序列具有70%以上同源性,且编码相同功能蛋白质的DNA序列。
在本发明的另一方面,还提供了一种载体,它包含上述编码特异靶向性药物的核酸分子。
在本发明的另一方面,还提供了一种用上述载体转化的宿主细胞。
在本发明的另一方面,还提供了一种药物组合物,该组合物含有安全有效量的特异靶向性药物和药学上可接受的载体。
本发明还提供了特异靶向性药物在制备治疗肝脏局域性疾病的药物中的应用。
较佳地,所述肝脏局域性疾病包括病毒性肝炎、肝硬化及肝脏肿瘤。
在本发明中,X可来源于具有肝脏特异性或相对特异性感染的病毒的蛋白,这些病毒包括人甲(Hepatitis A Virus,HAV)、乙(Hepatitis B Virus,HBV)、丙(HepatitisC Virus,HCV)、丁(Hepatitis D Virus,HDV)、戊(Hepatitis E Virus,HEV)以及其他型人类肝炎病毒、鸭肝炎病毒(Duck hepatiris virus,DHV)、土拨鼠肝炎病毒(WHV)、旱獭乙肝病毒(WHBV)、地松鼠肝炎病毒(GSHV)、长毛猴肝炎病毒(WMHV)、灰苍鹭乙型肝炎病毒(HHBV)、雪鹅肝炎病毒(SGHV)以及其他动物嗜肝病毒、以及其他具有肝脏特异性或相对特异性感染的病毒。本发明中的X优选地来源于人HBV、HCV、HAV病毒及其他人嗜肝病毒,进一步优选地来源于人HBV表面蛋白及其他介导或辅助人HBV特异性感染肝细胞的HBV病毒蛋白、人HCV病毒E1和E2蛋白及其他介导或辅助人HCV特异性感染肝细胞的HCV病毒蛋白、人HAV病毒VP1、VP2、VP3、VP4蛋白及其他介导或辅助人HAV特异性感染肝细胞的HAV病毒蛋白、以及其他介导或辅助人嗜肝病毒特异性感染肝细胞的嗜肝病毒蛋白。本发明中的X还包括能结合肝细胞表面特异或相对特异表达蛋白的多肽(天然序列或人工序列)或基团,这些在肝细胞表面特异或相对特异表达的蛋白包括CD81、低密度脂蛋白受体(low-densitylipoprotein receptor,LDL-R)、氨基葡糖多聚糖(glycosaminoglycans,GAG)、多聚人血清白蛋白(PHSA)、修饰的血清蛋白(modified serum albumin,MSA)、IgA受体、HBV结合因子(HBV BF)、p80、羧基肽酶D(gp180)、B类I型清道夫受体(scavengerreceptor class B type I,SR-BI)、甘露糖结合的凝血素DC SIGN(mannose bindinglectins DC SIGN)、L SIGN、无唾液酸糖蛋白受体(asialoglycoprotein receptor,ASGPr)、HAV细胞受体1(HAV cellular receptor 1,HAVcr-1)及其他在肝细胞表面特异或相对特异表达的蛋白。本发明中的一个实施例中,X来源于人HBV的病毒蛋白,优选地来源于人HBV的表面大蛋白,进一步地优选来源于HBV表面大蛋白Pre-S1区,其序列可进一步优选地自N和/或C末端缩短0至119个氨基酸,尤其优选X包含SEQ ID:1或与该序列具有0.1%至99.9%同源性的氨基酸序列,同时也包括来源于不同基因型(包括A至H基因型)和血清型(包括ayw1、ayw2、ayw3、ayw4、ayr、adw2、adw4、adrq+、adrq-)表面大蛋白序列和突变序列。在本发明的一个优选方案中,X特别优选地采用如SEQ ID NO:3所示的氨基酸序列。
本发明中X任何部分或末端可被优选地修饰,这些修饰包括在其N和/或C末端添加1至1000个氨基酸组成的多肽序列、在X的任何部分糖基化等化学修饰,较优选地SEQ ID NO:7的第13位氨基酸甘氨酸或本发明所包含其他序列所对应的氨基酸带有的疏水基团,这些疏水基团优选地具有4个以上碳原子的饱和或不饱和脂肪酸的丙烯残基,更优选的是豆蔻酸、棕榈酸、硬脂酸、油酸、亚油酸或花生四烯酸。疏水基团另外还优选胆固醇及其类似基团。在本发明的一个优选方案中,SEQ ID NO:6和SEQ ID NO:7的第13位氨基酸甘氨酸经豆蔻酰化(myristoylation)修饰。本发明中X的任何氨基酸残基可被替换,在一个优选方案中,SEQ ID NO:6的第15位氨基酸N(天冬酰氨)可被氨基酸Q(谷氨酰氨)替代。
本发明中的L为X与Y之间的任何连接(可完全缺失,使X与Y直接连接),这些连接包括氨基酸、多肽、蛋白质、化学键、核酸(DNA或RNA)、偶联剂(包括硫醋类、碳化二亚酰胺、琥珀酰亚胺酯类、二异氰酸酯(例如甲苯-2,6-二异氰酸酯)、谷二醛(gluteraldehydes)、重氮苯和六亚甲基二胺类(例如双-(对重氮苯甲酰基)-乙二胺)、亚氨酸酯类的双功能化衍生物(例如己二酰亚胺酸二甲酯)、双活性氟化合物(例如1,5-二氟-2,4-二硝基苯)、N-琉拍酞亚胺基-3--(2-吡啶基二硫代)丙酸(SPDP)、1-乙基-3-(3-二甲基氨基-丙基)碳化二亚胺盐酸盐(EDC)、4-琥珀酰亚胺基氧基羰基-α-甲基-α(2-吡啶基-二硫代)-甲苯(SMPT)以及其他偶联剂),以及其他用于生物分子之间的连接。优选地L为多肽连接,较优选地含有丝氨酸、甘氨酸、丙氨酸、苏氨酸等柔性氨基酸组成的多肽链,更优选地L为含有1至999个氨基酸的多肽链。在本发明的一个优选方案中,L为SEQ ID NO:4所示的多肽链。
本发明中Y表示具有药理或生理作用的药物或基团,优选地Y为对肝细胞、肝肿瘤细胞、肝细胞内病毒或肝脏内的细胞、肿瘤细胞及病原微生物具有药理或生理作用的药物或基团。Y包括蛋白质、多肽、细胞毒性小分子药物、放射性药物及其他药物,较优选地Y为对肝细胞、肝肿瘤细胞、肝细胞内病毒或肝脏内的细胞、肿瘤细胞及病原微生物具有药理或生理作用的蛋白质,包括细胞因子、毒性蛋白,更优选地Y为细胞因子,包括干扰素(interferon,IFN)、白细胞介素(包括白细胞介素1、白细胞介素2至白细胞介素100)、生长因子(包括肝细胞生长因子、肝细胞增殖素、肝生长抑制因子、肝促分化因子、促肝细胞生长素、肝素结合生长因子、纤维母细胞生长因子、表皮生长因子、血管内皮生长因子、角蛋白细胞生长因子、神经生长因、胰岛素样生长因子、血小板衍生生长因子、转化生长因子、干细胞因子、生长激素、肿瘤特异性生长因子、成纤维细胞生长因子)、集落刺激因子(包括粒细胞集落刺激因子、巨噬细胞集落刺激因子、粒细胞-巨噬细胞集落刺激因子、红细胞生成素、干细胞生成因子、多能集落刺激因子)、趋化因子(包括趋化因子α、β、γ、δ)及这些细胞因子的突变体和人工设计序列。尤其优选地Y为干扰素,包括IFNα、β、γ、ω、κ、τ、δ及其突变体和人工设计序列。特别优选地Y为干扰素α,包括IFNα-1a、α-1b、α-2a、α-2b其突变体和人工设计干扰素(包括INFERGEN及其他复合干扰素(consensus interferon),以及其他具有干扰素活性的突变体和人工设计的干扰素)。在本发明的一个优选方案中,Y为IFNα-2b(SEQ ID NO:5)或其突变体。本发明的Y包括与SEQ ID NO:5具有大于50%同源性的氨基酸序列。Y的任何部分或末端可被修饰,这些修饰包括在其N和/或C末端添加1至1000个氨基酸组成的多肽序列、在Y的任何部分糖基化、去糖基化、聚乙二醇(PEG)及其他化学修饰。
本发明中X和Y的位置可颠倒,X、L、Y之间可进行单一的或多倍的排列组合,例如但不限于形成X-L-Y-L-X、Y-X-Y等形式。多倍排列组合中的各X或Y可相同或不同。在本发明中的一个优选方案中,采用X-L-Y结构,X来源于人乙型肝炎病毒表面大蛋白Pre-S1区多肽,L为柔性氨基酸链接,Y为干扰素α-2b,从而发明了特异靶向性干扰素,特别优选氨基酸序列见SEQ ID NO:7,其中X和Y分别位于序列的N和C末端,该特异靶向性IFN,能在延长IFN半衰期的同时,将IFN靶向到肝脏,提高了IFN在肝脏的局部浓度,且在增强IFN治疗肝部疾病疗效的同时降低肝脏外IFN引起的不良反应。。
本发明的特异靶向性药物可采用核酸序列编码(包括DNA和RNA序列),优选地采用DNA序列编码。在本发明的一个实施例中,优选的氨基酸序列见SEQ ID NO:7,其对应的DNA编码序列为SEQ ID NO:8,本发明包含与SEQ ID NO:8编码相同氨基酸序列的简并DNA序列。在保持简并性条件下优选地按照细菌、酵母细胞、动物细胞、植物细胞和昆虫细胞及其他细胞或生物喜用密码子规律调整DNA编码序列,使DNA编码序列更好地在细菌、酵母细胞、动物细胞、植物细胞、昆虫细胞及其他细胞或生物中表达。本发明优选地采用酵母细胞喜用密码子编码靶向性干扰素SEQ ID NO:7,其相应的DNA序列为SEQ ID NO:9。进一步优选地,本发明对SEQ ID NO:6中的潜在糖基化为点进行替换,以避免在酵母表达过程中特异靶向性干扰素被过分糖基化而影响特异靶向性干扰素的活性,替换后的序列为SEQ ID NO:7。其他位点经替换而形成的序列为本发明的一部分,本发明包含与SEQ ID NO:8和SEQ ID NO:9具有大于50%同源性的DNA序列。
本发明中的载体包括细菌表达载体、酵母表达载体、动物细胞表达载体、植物细胞表达载体、昆虫细胞表达载体、病毒载体及其他表达载体。在本发明的一个优选方案中将编码特异靶向性药物的DNA片段克隆入酵母分泌性表达和胞内表达载体,这些载体包括pPIC9、pPIC9K、pPIC3、pPIC3K、pA0804、pA0815、pHIL-S1、pHIL-D2、pHW010、pPICZ、pPICZα、pGAPZ、pGAPZα、pYAM7SP6、pMEN6K、pMEX9K及其他酵母表达载体。更优选地将编码特异靶向性药物的DNA片段克隆入pPIC9K酵母表达载体。在本发明的一个实施例中,化学合成的特异靶向性干扰素编码DNA片段克隆入pPIC9K酵母表达载体,形成重组酵母表达载体pPIC9K-IFN(图3B)。
本发明还包含由含有编码特异靶向性药物DNA序列表达载体转化的细胞宿主和动植物宿主,这些细胞宿主包括细菌、酵母菌、动物细胞、植物细胞、昆虫细胞,其中的细菌包括大肠杆菌DH5α、BL21、JM83、JM107、JM109、C600、KS476、JM109、MC1061、YA21、YK537;动物宿主包括牛、羊、猪;植物宿主包括番茄、马铃薯、香蕉。在本发明的一个优选方案中,包含由含有特异靶向性药物DNA序列的表达载体转化的酵母菌,这些酵母菌包括巴斯德毕赤氏母(Pichia pastoris)、博伊丁假丝酵母(Candida boidinii)、汉逊酵母(Hansenula)、球拟酵母(Torulopsis)、酿酒酵母(Saccharomyces cerevisiae),优选巴斯德毕赤酵母和多形汉逊酵母,尤其优选营养缺陷型巴斯德毕赤酵母菌株GS115(NRRLY-15851)、GS190(NRRLY-18014)、PPFI(NRRLY-18017)、KM71和蛋白酶缺陷型巴斯德毕赤酵母菌株SMD 1168,特别优选巴斯德毕赤酵母菌株GS115。在本发明的一个实施方案中,重组的酵母表达载体pPIC9K-IFN经线性化后转化酵母菌GS115,经筛选获得整合有特异靶向性干扰素编码DNA序列的GS115菌株。
整合有特异靶向性药物编码DNA序列的宿主,经过培养或发酵,表达特异靶向性药物,经纯化可获得特异靶向性药物。在本发明的一个实施例中,整合有特异靶向性干扰素编码DNA序列的宿主GS115菌株经发酵表达特异靶向性干扰素蛋白。这些含有特异靶向性干扰素蛋白的发酵上清经纯化后获得特异靶向性干扰素纯蛋白。特异靶向性干扰素按照中国生物制品规程(中国生物制品标准化委员会编.[M].北京:化学工业出版社,2000,373-375.)进行活性测定,表明目的蛋白具有良好的抗病毒活性(0.9×108IU/mg)。同时,特异靶向性干扰素对人肝细胞具有明显的特异性亲和作用。
本发明中所述药物组合物含有安全有效量的特异靶向性药物和药学上可接受的载体,这类载体包括淀粉、糊精、蔗糖、乳糖、纤维素类、硬脂酸镁、吐温-80、卡波姆、甲基纤维素、羧甲基纤维素钠、海藻酸钠、甘油、明胶、聚乙二醇、硫柳汞、尼泊金丙酯、尼泊金甲酯、尼泊金乙酯、三氯叔丁醇、苯甲酸钠、硼砂、新洁尔灭、山梨醇、丙二醇、异丙醇、月桂氮桌酮,异丙醇/丙二醇、异丙醇/丙二醇、三乙醇胺、氢氧化钠凡士林、硬脂酸、液状石蜡、羊毛脂、十八醇、十六醇、单硬脂酸甘油酯、月桂醇硫酸钠、司盘60、平平加、甘露醇、山梨醇及其他药物载体。制剂方式包括注射剂、冷冻干燥注射剂、脂质体注射剂、靶向给药注射剂、片剂、胶囊剂、喷雾剂、凝胶剂、凝胶吸入剂、口服液、混悬剂、冲剂、贴剂、丸剂、散剂、注射剂、输液剂、栓剂、缓释制剂、控释制剂及其他制剂。
本发明还包括特异靶向性药物在制备治疗肝炎(包括甲、乙、丙、丁、戊及其他型病毒性肝炎)、肝硬化、肝脏肿瘤(原发肿瘤及转移肿瘤)及其他肝脏疾病的药物中的应用。
本发明的特异靶向性药物利用嗜肝病毒的嗜肝特异性分子机制,将介导肝细胞特异性感染的病毒蛋白或多肽与治疗性分子相连接,产生的特异靶向性药物可对病毒性肝炎、肝硬化、肝脏肿瘤等肝脏疾病进行靶向治疗,在增强药物疗效的同时又降低药物对肝脏以外器官造成的不良反应。
附图说明
图1特异靶向性干扰素氨基酸序列N连接糖基化位点分析;
图2编码特异靶向性干扰素DNA序列的酵母菌密码子偏好性分析;
图3pPIC9K、pPIC9K-IFN图谱及KEX-2、STE-13酵母内源蛋白酶加工位点;
图4特异靶向性干扰素SDS-PAGE电泳图及HPLC纯度分析图;
图5FITC标记的特异靶向性干扰素及rIFNα-2b对人肝细胞亲和力比较。
具体实施方式
下面结合附图和实施例对本发明作进一步详细的说明。
以下实施例仅用于说明本发明而不用于限制本发明的范围。实施例中未注明具体条件的实验方法,通常按照常规条件,例如Sambrook等人,分子克隆:实验室手册(New York:Cold Spring Harbor Laboratory Press,1989)中所述的条件,或按照制造厂商所建议的条件。
实施例1特异靶向性干扰素氨基酸序列的设计
1.X序列选择HBV毒株FMC#97表面大蛋白第1到50氨基酸序列(SEQ ID NO:3),该序列包括被广泛证实的与肝细胞表面特异性结合并介导HBV感染肝细胞的关键序列。
2.L选择由柔性氨基酸组成的序列(SEQ ID NO:4),以减少X与Y之间在蛋白构象和功能上的相互影响。
3.Y序列选择IFNα-2b全长氨基酸序列(SEQ ID NO:5)。
4.X和Y分别位于L序列的N末端和C末端,形成的整体序列见SEQ ID NO:6。
5.对SEQ ID NO:6进行糖基化位点分析(见图1),其中第15位氨基酸天冬酰氨为可能的N连接糖基化修饰位点,将其进行类似氨基酸突变替换(15N→Q),以消除特异靶向性干扰素在酵母表达过程中出现过度糖基化而影响IFN和Pre-S1的功能活性,形成的最终特异靶向性干扰素氨基酸序列为SEQ ID NO:7。
实施例2编码特异靶向性干扰素的DNA序列的设计
1.选择毕赤酵母作为特异靶向性干扰素的表达系统。毕赤酵母是一种用于外源蛋白表达最成功的真核表达系统(Cereghino J L,Cregg J M.Heterologous proteinexpression in the methylotrophic yeast Pichia pastoris[J].FEMS MicrobiolRev,2000,24(1):45-66.)。既具有原核表达系统繁殖迅速、费用低廉及操作方便的特点,又具有外源蛋白质加工折叠正确和适度糖基化的真核表达系统优点。因此越来越广泛地用于蛋白质的大量表达,目前已有200多种蛋白在该表达系统中得以表达(Cregg JM,Cereghino JL,Shi JY,et al.Recombinant protein expression inPichia pastoris[J].Mol Biotechnol,2000,16(1):23-52.)。毕赤酵母具有胞内表达和分泌表达两种表达方式,其中分泌表达方式因其表达量高、糖基化完全、二硫键和高级结构形成正确、后续分离纯化简便而备受青睐。
2.进行特异靶向性干扰素编码基因设计时考虑如下原则:1)特异靶向性干扰素编码基因尽可能选用巴斯德毕赤酵母醇氧化酶(AOX 1)基因偏爱的密码子,降低该基因中毕赤酵母罕用密码子的比例;2)消除特异靶向性干扰素基因内部可能出现的复杂二级结构(包括重复结构、互补结构、发夹结构及大片段的反向回文结构等);3)消除特异靶向性干扰素基因内部不适宜基因操作的限制性内切酶位点;4)在特异靶向性干扰素基因内部尽量减少连续的G-C配对,增加毕赤酵母偏爱的A-T配对,但避免出现基因G+C%失调。
3.特异靶向性干扰素SEQ ID NO:7对应的自然DNA序列为SEQ ID NO:8,其酵母密码子偏好分析见图2A。经过以上原则的重新设计,用于酵母表达载体的特异靶向性干扰素DNA序列为SEQ ID NO:9,其酵母密码子偏好分析见图2B,未见偏好小于10%的稀有密码子。
实施例3特异靶向性干扰素酵母表达载体的构建
1.选择pPIC9K为特异靶向性干扰素的酵母表达载体。pPIC9K是Invitrogen公司推出的多拷贝分泌型表达载体,大小为9.3kb(如图3A)。该载体含有大肠杆菌复制起点Col E1和氨苄青霉素及卡那霉素两个抗性基因,其中卡那霉素抗性基因还可以使毕赤酵母对G418产生抗性,可用于多拷贝插入的筛选。载体中使用醇氧化酶基因的启动子(pAOX1)做为诱导型启动子,该启动子受葡萄糖抑制,甲醇诱导后才开始转录和翻译,非常适合于外源基因的表达。pPIC9K利用a交配因子引导序列的分泌信号将目的基因产物分泌至胞外。由于毕赤酵母本身仅将总量5%的蛋白分泌至胞外,因此对分泌表达的蛋白进行分离纯化极为方便。该载体在a交配因子引导序列与目的蛋白之间引入了酵母内源性蛋白酶KEX-2和STE-13加工位点(图3C),使表达的目的产物经酵母内源性蛋白酶加工后,可以直接获得N末端无a交配因子引导序列的目的蛋白。
2.在设计的特异靶向性干扰素DNA序列(SEQ ID NO:9)的5’和3’两端根据需要分别加入EcoR I、Not I酶切位点粘性末端。化学合成特异靶向性干扰素DNA序列的正链和负链,退火后将特异靶向性干扰素DNA序列克隆入pPIC9K的EcoR I、NotI酶切位点。将链接后的载体转染大肠杆菌中扩增,挑取单克隆菌落,抽提质粒测序鉴定正确连入的重组pPIC9K,即pPIC9K-IFN(图3B)。
实施例4特异靶向性干扰素的酵母表达
1.酵母表达载体分为附加体型与整合体型两种宿主携带方式。附加体型的重组载体存在于酵母的细胞质内,重组质粒在酵母宿主细胞芽殖分裂、世系传代中容易丢失,因而难以用于工业化大型发酵罐的大生产。整合体型表达载体是以线形化质粒或环形质粒形式通过同源重组方法整合到酵母的基因组内(单拷贝或多拷贝整合),然后随着酵母宿主菌染色体的复制而复制,外源目的基因在酵母世系传代趋于稳定,适合用工业化大型发酵罐来进行发酵生产。pPIC9K即为多拷贝整合体型酵母表达载
2.重组酵母表达载体pPIC9K-IFN经酶切线性化后,电转化法转化毕赤酵母宿主菌GS115,其方法参照Invitrogen毕赤酵母实验手册。
3.重组酵母克隆的筛选,其筛选方法参照Invitrogen毕赤酵母实验手册。
4.特异靶向性干扰素的诱导表达:将筛选出的重组克隆接种于5ml BMGY培养基中,30℃ 300r/min培养至OD600 4.0至6.0。室温6000r/min离心4min收集菌体,用BMMY悬浮并稀释至OD600 1.0,30℃ 300r/min每12h补充甲醇至0.5%诱导培养48h后收集培养上清,SDS-PAGE检测蛋白表达。
5.结果显示,电转化后的毕赤酵母GS115经过筛选得到1个最高表达的转化酵母宿主菌株(GS115/pPIC9K-IFN)。
实施例5特异靶向性干扰素的分离纯化
1.在本发明中,发酵培养酵母工程菌(GS115/pPIC9K-IFN)的种子培养基和发酵培养基(发酵罐用)均为已知培养基,如:YPD平板、BMGY液体培养基、基础盐(合成)培养基(参见“High Cell-Density Fermentation in Pichia Protocols”,editedby David R.Higgins and James M.Cregg,Vol.103,107-120,1998)和FM22培养基;酵母工程菌(GS115/pPIC9K-IFN)的种子培养、发酵罐培养、外源蛋白诱导表达的方法,均为Pichiafermentation process guidelines(Invitrogen Corporation,2002)上提到的方法或在此基础上修改的方法。
2.GS115/pPIC9K-IFN高表达酵母经种子培养、发酵罐培养、外源蛋白诱导表达后,将诱导发酵48h的菌液10,000r/min离心10min后,取上清用0.45um滤膜过滤,上清液经Hiprep疏水层析、Blue Sepharose FF亲和层析、Superdex 75凝胶过滤层析纯化。
3.GS115/pPIC9K-IFN高表达酵母经发酵培养后发酵液内特异靶向性干扰素经纯化后,SDS-PAGE(图4A)所示分子量约27kDa处蛋白条带即为重组酵母表达的特异靶向性干扰素蛋白,HPLC鉴定纯度大于95%(图4B)。
实施例6特异靶向性干扰素的干扰素活性检测
1.通过WISH-VSV法测定特异靶向性干扰素的干扰素活性。
2.将人羊膜WISH细胞悬液接种于96孔板,每孔3.5×1011cell/100ul,37℃、5%CO2条件下培养4-6h,取纯化的特异靶向性干扰素做系列稀释后每孔加入100ul,37℃培养24h后吸弃上清,用含3%牛血清的DMEM培养基稀释水泡性口炎病毒(VSV)至工作浓度(250TCID50/ml),每孔加入100ul以感染WISH细胞,继续培养24h。
3.每孔加入200ul0.5%的结晶紫液(0.5g结晶紫、0.85g NaCl溶于50ml无水乙醇、3ml甲醇、47ml水),置37℃15min,漂洗残余染料,每孔加入200ul脱色液溶解细胞内染料,测定每孔的A578nm吸收值,以rHuIFNα-2b为参考品按下列公式计算特异靶向性干扰素效价:
待检样品效价=标准品效价×(待检样品预稀释倍数/标准品预稀释倍数)×(待检样品半效稀释倍数/标准品半效稀释倍数)
其中待检样品半效稀释倍数,即从特异靶向性干扰素溶液至相当于标准品50%最大效应点的稀释倍数。
4.结果表明特异靶向性干扰素比活达到0.9×108IU/mg。
实施例7特异靶向性干扰素肝细胞靶向效应的检测
1.人原代肝细胞的培养:非HBV相关的肝癌患者外科手术肿瘤切除物相邻的正常组织,按文献所述方法进行分离〔Guguen-Guillouzo,C.,和A.Guillouzo,1986.Methods for preparation of adult and fetal hepatocytes,第1-12页,在A.Guillouzo和C.Guguen-Guillouzo编辑的“Isolated and cultured hepatocytes”中.Les E′ditions INSERM Paris,John Libbey and Co.,Ltd.,英国伦敦〕,培养于添加了3.5×10-6M氢化可的松琥珀酸单酯(hydrocortisone hemisuccinate)、2%二甲基亚亚砜、5%人血清和5%胎牛血清的H培养基中。
2.特异靶向性干扰素和rHuIFNα-2b蛋白的FITC标记。将蛋白溶液置于碳酸盐缓冲液(0.16M Na2CO3,0.33M NaHCO3,pH9.5)中透析过夜。FITC溶于DMSO中,终浓度为1mg/ml。将透析过的蛋白溶液置于小瓶中,按250μg FITC/mg蛋白的比例,边搅拌边滴加适量的FITC溶液。于4℃,避光搅拌结合12hr。将Sephadex G25充分膨胀后,仔细装柱,柱长度为15cm,直径为0.9cm,柱体积为9.5ml。装柱完毕后,于凝胶表面覆盖一层滤纸,用PBS充分洗柱。将标记的蛋白混合液加入柱中,上样体积不超过柱床体积的10%。用PBS洗脱,收集第一个洗脱峰,检测各收集管的A280和A495。计算荧光素与蛋白质结合比率(F/P),计算公式为F/P=2.87×A495/(A280-0.35×A495)。F/P值为2~4的组份混合,PBS透洗后即为FITC标记好的蛋白。
3.人原代肝细胞于12孔培养板中培养,每孔约106细胞与FITC标记的特异靶向性干扰素或rHuIFNα-2b蛋白孵育60分钟。移除上清后PBS漂洗细胞2次,经1%甲醛固定后于荧光显微镜488nm下观察。可见特异靶向性干扰素(图5A)较rHuIFNα-2b(图5B)对肝细胞具有更高的亲和力。
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Claims (20)
1.一种特异靶向性药物,其特征在于,它具有通式X-L-Y,其中,
X表示氨基酸序列,该序列包含:(a)来源于具有肝脏特异性或相对特异性感染病毒的蛋白的氨基酸序列,(b)由(a)的序列发生一个或多个氨基酸残基的置换、缺失、插入或添加且与(a)具有相同活性的氨基酸序列,所述病毒蛋白与细胞感染受体或辅受体相结合,并介导或辅助病毒的感染;
L表示X与Y之间的任一连接,该连接可缺失;
Y表示对正常细胞、病理状态下细胞、受感染细胞、肿瘤细胞及病原微生物具有药理或生理作用的药物或基团;
所述X和Y的位置可颠倒,X、L、Y之间可进行单一或多倍的排列组合,且多倍排列组合中的各X或Y可相同或不同。
2.如权利要求1所述的特异靶向性药物,其特征在于,所述具有肝脏特异性或相对特异性感染病毒包括甲型肝炎病毒、乙型肝炎病毒、丙型肝炎病毒、丁型肝炎病毒、戊型肝炎病毒及未分型肝炎病毒。
3.如权利要求1所述的特异靶向性药物,其特征在于,所述Y是对正常肝细胞、病理状态下肝细胞、受感染肝细胞、肝肿瘤细胞及肝细胞内病毒或病原微生物具有药理或生理作用的药物,包括蛋白质、多肽、细胞毒性药物、小分子药物及放射性药物。
4.如权利要求3所述的特异靶向性药物,其特征在于,所述蛋白质药物包括细胞因子、干扰素、白细胞介素、生长因子、集落刺激因子、趋化因子及该类蛋白质药物的突变体。
5.如权利要求1或2所述的特异靶向性药物,其特征在于,所述X序列包含:人乙型肝炎病毒表面大蛋白Pre-S1的多肽,或其保守性变异多肽、或其活性片段,或其活性衍生物。
6.如权利要求5所述的特异靶向性药物,其特征在于,所述X序列包含:具有SEQ ID NO:1氨基酸序列的人乙型肝炎病毒表面大蛋白Pre-S1多肽,或其保守性变异多肽、或其活性片段,或其活性衍生物。
7.如权利要求6所述的特异靶向性药物,其特征在于,所述X序列选自下组:
(a)具有SEQ ID NO:1氨基酸序列的多肽;
(b)将SEQ ID NO:1氨基酸序列经过一个或几个氨基酸残基的置换、缺失、插入或添加且具有与SEQ ID NO:1氨基酸序列相同活性的由(a)衍生的多肽。
8.如权利要求7所述的特异靶向性药物,其特征在于,所述X序列为(b)多肽,优选为具有SEQ ID NO:3氨基酸序列的多肽。
9.如权利要求1所述的特异靶向性药物,其特征在于,所述L为X与Y之间的氨基酸连接。
10.如权利要求3或4所述的特异靶向性药物,其特征在于,所述Y包含:干扰素α、干扰素β、干扰素γ、干扰素ω、干扰素κ、干扰素τ、干扰素δ,或其保守性变异蛋白质、或其活性片段,或其活性衍生物。
11.如权利要求10所述的特异靶向性药物,其特征在于,所述Y选自下组:
(a)具有SEQ ID NO:2氨基酸序列的干扰素α-2b;
(b)由(a)的蛋白发生一个或多个氨基酸残基的置换、缺失、插入或添加且与(a)的干扰素α-2b具有相同活性的衍生蛋白质。
12.如权利要求11所述的特异靶向性药物,其特征在于,所述Y为(b)蛋白质,优选为具有SEQ ID NO:5氨基酸序列的干扰素α-2b。
13.如权利要求9所述的特异靶向性药物,其特征在于,所述L为主要由G(甘氨酸)、A(丙氨酸)、S(丝氨酸)和T(苏氨酸)四种氨基酸组成的氨基酸序列。
14.如权利要求1至13中的任一项所述的特异靶向性药物,其特征在于,所述药物具有SEQ ID NO:6的氨基酸序列,优选SEQ ID NO:6氨基酸序列第15位氨基酸N(天冬酰氨)被氨基酸Q(谷氨酰氨)替换,产生SEQ ID NO:7氨基酸序列。
15.一种核酸分子,其特征在于,它编码权利要求1至14中任一项所述的特异靶向性药物的氨基酸序列。
16.如权利要求15所述的核酸分子,其特征在于,它包括下列核苷酸序列之一:
(1)序列表中SEQ ID NO:8或SEQ ID NO:9的DNA序列;
(2)编码序列表中SEQ ID NO:7氨基酸序列的多核苷酸;
(3)与序列表中SEQ ID NO:8或SEQ ID NO:9的DNA序列具有70%以上同源性,且编码相同功能蛋白质的DNA序列。
17.一种载体,其特征在于,它包含权利要求15或16所述的核酸分子。
18.一种用权利要求17所述的载体转化的宿主细胞。
19.一种药物组合物,其特征在于,它含有安全有效量的权利要求1至14中任一项所述的特异靶向性药物和药学上可接受的载体。
20.权利要求1至14中任一项所述的特异靶向性药物在制备治疗肝脏局域性疾病的药物中的应用,所述肝脏局域性疾病包括病毒性肝炎、肝硬化及肝脏肿瘤。
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