CN100390201C - 具有增强红细胞生成素体内活性的融合蛋白 - Google Patents
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Abstract
本发明涉及具有增强红细胞生成素体内活性的融合蛋白,其中将血小板生成素的羧基端肽片段与人红细胞生成素的羧基端融合。该融合蛋白由于碳水化合物含量增加显著提高了体内半寿期,并且不损失红细胞生成素的固有活性,当给人体施用时不会带来任何抗原性。
Description
技术领域
本发明涉及具有增强红细胞生成素(下简称EPO)体内活性的融合蛋白,所述EPO是治疗贫血症的新药。具体而言,通过将EPO分子与具有延长半寿期活性并衍生自人体的一定肽融合,本发明涉及具有高度增强红细胞生成素体内半寿期和活性的融合蛋白。
背景技术
EPO为糖蛋白,分子量30,000-34,000,是促进红细胞生成和分化的因子。该蛋白与红细胞前体细胞上的受体结合后导致细胞内钙离子浓度降低、DNA生物合成增加、刺激血红蛋白形成等。所述EPO能用于治疗肾衰竭贫血、早产婴儿贫血、甲状腺功能减退贫血以及营养不良贫血等。重组人EPO的临床使用与日俱增。但是由于其半寿期短,每周平均需要施用三次,这种使用可带来某些不便和高额费用。因而,如果EPO的体内活性能维持长时间,则可大大降低施用EPO的次数。
EPO功效与其体内半寿期成正比。已知EPO体内半寿期与位于EPO碳水化合物链末端的唾液酸含量相关。因此,EPO功效高度依赖于碳水化合物链的存在。由于碳水化合物的形式在各种表达EPO的细胞中有不同表现,因此相同糖蛋白在不同细胞中表达时可有不同的碳水化合物结构。尽管最近已表明一些细菌能添加碳水化合物链,但已知典型细菌如大肠杆菌(E.coli)就不会。E.coli中表达的蛋白不含有碳水化合物链,因此衍生自E.coli的EPO也不含有碳水化合物链,其在体外表现出活性,但在体内却没有活性。这是因为去糖基化的EPO从人体中很快消除,半寿期极短。总之,碳水化合物链在EPO活性中发挥极其重要的作用。
已进行了许多研究来增强EPO的活性。主要途径是通过EPO基因上的诱变取代一些EPO氨基酸。例如,Amgen公司提交的题目为“红细胞生成素类似物”的专利申请PCT/US94/09257公开了通过诱变增加碳水化合物含量来提高EPO体内半寿期的方法。还通过形成EPO二聚体来试图提高EPO的体内半寿期。参见A.J.Sytkowski等,J.B.C.274(35):24773-24778。此外,另一已知方法是将新氨基酸、肽或蛋白片段与EPO分子通过基因工程方式融合以及提高EPO的碳水化合物含量,即唾液酸含量,从而增强体内EPO活性。然而,并非所有氨基酸、肽或杂合蛋白片段能用于此目的。在大多数情况下,这些修饰可导致蛋白固有活性的降低或损失,并且体内使用时可带来抗原性问题。
虽然与EPO无关,融合蛋白或嵌合蛋白已用于研究例如一种性激素促卵泡激素。参见Furuhashi等,1995,Mol.Endocrinol.。不过,由于采用基因工程方法进行蛋白修饰存在一些风险,这些方法还未应用到工业上。即,在大多数情况下,没有专业技能不易获得靶蛋白,与之相反,通过添加或取代以新氨基酸则可降低或丧失蛋白固有活性。
发明内容
本发明人通过将新氨基酸、肽或蛋白片段与EPO分子融合并由此提高其碳水化合物含量,已广泛研究了增强EPO体内活性的新方法。结果本发明人发现,将已在人体内存在的血小板生成素(下简称TPO)的羧基端肽(下简称CTP)与EPO的羧基端融合,可得到EPO融合蛋白,由于许多氨基酸增加糖基化位点,该融合蛋白具有高度增强的体内半寿期同时又不损失EPO的固有活性,并且给人体施用时不会导致任何抗原性。由此,本发明人完成了本发明。
因此,本发明目的是提供一种融合蛋白,该融合蛋白具有增强的人EPO体内活性并含有与人EPO在其羧基端相融合的TPO的CTP。
本发明的另一个目的是提供编码该融合蛋白的核酸、含有该核酸的重组载体以及被该重组载体转化了的宿主细胞系。
本发明的进一步目的是通过培养转化的细胞系提供制备具有增强人EPO体内活性的融合蛋白的方法。
首先,本发明涉及一种融合蛋白,该融合蛋白具有增强的人EPO体内活性并含有与人EPO在其羧基端相融合的TPO的CTP。CTP优选包含对应于位置176-353氨基酸(下简称LTP)的SEQ ID No.1氨基酸序列或其部分,尤其包含对应于位置337-353氨基酸(下简称STP)的SEQ ID No.2氨基酸序列。
特别地,根据本发明的融合蛋白包含SEQ ID No.3或4的氨基酸序列。
其次,本发明涉及编码融合蛋白的核酸、含有该核酸的重组载体以及被该重组载体转化了的宿主细胞系,优选CHO细胞(中国仓鼠卵巢细胞)。
第三,本发明涉及通过培养转化的细胞系制备具有增强人EPO体内活性的融合蛋白的方法。
以下将更详细解释本发明。
附图简述
附图1a和1b表示TPO羧基端肽(LTP、STP)的核苷酸和氨基酸序列;
附图2aa和2ab表示EPO和肽LTP的融合蛋白ELTP的核苷酸和氨基酸序列,以及附图2b表示EPO和肽STP的融合蛋白ESTP的核苷酸和氨基酸序列;
附图3a和3b表示表达载体pcDNA-ELTP和pcDNA-ESTP制备过程的图解;
附图4为被表达的ELTP和ESTP的电泳照片;以及
附图5表示EPO、ELTP和ESTP的药代动力学结果。
发明最佳实施方式
本发明包含下列步骤:所需融合蛋白基因的制备和克隆,含有所需基因的表达载体的构建,动物细胞的转化,表达,纯化和生物分析。
(1)基因制备
采用EPO cDNA末端的互补引物(EP1和EP2),执行常规PCR技术(Bioneer公司的PCR PreMix Kit)从衍生自人胎儿肝脏的cDNA文库(Invitrogen公司)中可获得EPO cDNA。采用TPO cDNA末端的互补引物(T1和T2)以相同方式可获得TPO cDNA。
EP1:ATGGG GGCAC GAATG TCCTG CCTGG CTGG(SEQ IDNo.5)
EP2:GTCCC CTGTC CTGCA GGCCT(SEQ ID No.6)
T1:ATGGA TCTGA CTGAA TTGCT CCTC(SEQ ID No.7)
T2:TTACC CTTCC TGAGA CAGAT TCTGG GA(SEQ ID No.8)
由PCR获得的EPO cDNA和TPO cDNA分别克隆到克隆载体pGEM-T(Promega公司)中。然后将pGEM-EPO和pGEM-TPO测序并用作下列程序的模板。
以pGEM-TPO为模板,采用引物EL1和T2,通过PCR扩增,可获得本发明所用的TPO的CTP基因LTP。
EL1:GAGGC CTGCA GGACA GGGGA CGCCC CACCC ACCACAGCTG TCC(SEQ ID No.9)
引物EL1含有延伸至靠近EPO 3’端的限制性酶StuI位置的基因,以及同时含有LTP基因(TPO位置176-353的氨基酸)5’端的一部分。另一方面,以pGEM-EPO为模板,采用引物EP1和EP2,进行PCR扩增,只生成EPO基因。由此获得的EPO和LTP基因分别用限制性酶StuI处理。然后,将EPO和LTP基因片段连接,并在PCR程序中以连接产物为模板,采用引物EP11和L2,从而生成含有约1113bp(碱基对)的基因片段ELTP。
EP11:TAAGC TTATG GGGGT GCACG AATGT(SEQ ID No.10)
L2:TGGAT TCTTA CCCTT CCTGA GACAG ATTC(SEQ IDNo.11)
将该基因克隆到克隆载体pGEM-T中,然后测序(pGEM-ELTP,附图3a)。
进一步,本发明所用的STP基因可由合成和自身引导PCR程序获得。合成的基因片段为下述的ES1、S2、S3和上述的L2。
ES1:AGGGG AGGCC TGCAG GACAG GGGAC CCTCT TCTAA(SEQ ID No.12)
S2:GTGGG TGTAG GATGT GTTTA GAAGA GG(SEQ ID No.13)
S3:TACAC CCACT CCCAG AATCT GTCTC(SEQ ID No.14)
4种基因片段每种取出1μl(50pmol/μl),采用宝灵曼(BM)公司的高保真Taq系统进行PCR扩增。
将约50bp的基因片段(STP基因)在1%琼脂糖凝胶中鉴定。该基因编码TPO羧基端的17个氨基酸(位置337-353的氨基酸)(附图1)。
以pGEM-EPO为模板,采用引物EP11和EP2,进行PCR扩增,只生成EPO基因。以该EPO基因和STP基因同时作为模板,采用引物EP11和L2,经BM公司的高保真Taq系统进行PCR扩增,生成约630bp的所需融合基因即ESTP基因。将该基因克隆到克隆载体pGEM-T中,然后测序(pGEM-ESTP,附图3b)。
(2)表达载体构建
Invitrogen公司的pcDNA3.1载体用作表达载体。
将pcDNA3.1载体用限制性酶HindIII和BamHI处理生成线性载体,将pGEM-ELTP和pGEM-ESTP也分别用相同的限制性酶HindIII和BamHI处理。将消化的pcDNA3.1、ELTP和ESTP基因采用Qiagen提取试剂盒在琼脂糖凝胶上分离。各个基因连接后,将连接产物导入E.coli NM522中。将该转化的E.coli在LB-氨苄青霉素平板上过夜培养,从所形成的菌落中分离出质粒,并用限制性酶HindIII和BamHI处理。然后用1%琼脂糖凝胶电泳筛选出含有ELTP或ESTP基因的菌落。分别将这些质粒命名为pcDNA-ELTP和pcDNA-ESTP(附图3a和3b)。
(3)CHO细胞转化和表达
将CHO细胞(DG44)在60mm细胞培养皿中培养到40-80%汇合(1-4×105细胞/60mm培养皿)。将3μl的superfection试剂(BM公司)和97μl的细胞培养基(带有基质的α-MEM、无血清、无抗生素)混合均匀,并向其中加入pcDNA-ELTP(=0.1μg/μl,约2μg)和含有dhfr基因的载体pLTRdhfr26(ATCC37295,0.2μg)。室温下混合物反应5-10分钟,然后加入如上所制备的细胞中。一天后,用含有G418的培养基(无基质的α-MEM,10%的FBS)以500μg/ml的量更新培养基。然后用含有500μg/ml G418的G418培养基更新培养基7-10天,在此期间,无G418抗性基因的细胞以及阴性对照细胞被完全杀死。将G418培养基上所筛选出的细胞培养充分,并采用BM公司的EPO ELISA试剂盒鉴定表达的ELTP蛋白。对ESTP表达载体使用相同方法,而后以相同方式鉴定表达的ESTP融合蛋白。
(4)被表达的ELTP和ESTP的纯化
采用抗EPO单克隆抗体(R&D公司)按如下方法制备用于分离和纯化的亲和树脂:
将0.3g CNBr活化的琼脂糖凝胶4B在1mM HCl中溶胀20分钟,然后将树脂移至柱内,并用1mM HCl洗涤。用4ml偶联缓冲液(0.1MNaHCO3,0.5M NaCl,pH8.3)洗涤树脂,立即与含在4ml偶联缓冲液中的抗EPO单克隆抗体(500μg/瓶)混合,并在室温下震荡试管反应2小时。用封闭缓冲液(0.2M甘氨酸,pH8.0)更新后,震荡试管使树脂在室温下反应2小时。然后将树脂按序用6.5ml偶联缓冲液、6.5ml醋酸缓冲液(0.1M醋酸,0.5M NaCl,pH4)以及6.5ml偶联缓冲液洗涤。以如此获得的树脂制备柱子,并按如下所述进行纯化。
细胞在无血清培养基中培养一天后,采用Centriprep(Millipore,截留分子量10,000)将培养基浓缩约5倍。该浓缩液以20ml/小时流速装载到预先用PBS平衡过的柱上,并用PBS再次洗脱。将洗脱缓冲液(0.1M甘氨酸,pH2.8)施加到柱上,并将洗脱液立即用1M Tris滴定至pH7.5。用SDS-PAGE和银染分析,纯度至少为97%(附图4)。
(5)生物分析方法测定活性
在采用经苯肼处理的小鼠脾细胞的生物分析试验中,ELTP和ESTP表达并被适当纯化后,比EPO显示较高的活性。这表明ELTP和ESTP中的融合羧基端不能抑制EPO自身活性。
(6)药代动力学实验
对小鼠进行药代动力学实验以测定所制备的ELTP和ESTP是否真正延长了体内半寿期。将候选物质以20单位/小鼠的量静脉施用给4只小鼠。为了鉴定血液中的定时浓度,每间隔30分钟从小鼠中取出血液,并采用宝灵曼(BM)公司的EIA试剂盒测定浓度。在小鼠的药代动力学实验中,候选物质ELTP和ESTP比对照EPO显示长得多的半寿期(附图5)。
本发明将以下列实施例更具体地解释。但是应理解下列实施例旨在描述本发明,而不是以任何方式限制本发明的范围。
实施例1:基因制备
采用与EPO cDNA末端互补的引物EP1和EP2各50pmol,从人衍生的胎儿肝脏的cDNA文库(Invitrogen公司)中进行常规PCR(Bioneer公司的PCR PreMix试剂盒),从而获得EPO cDNA。采用与TPO cDNA末端互补的引物T1和T2以相同方式获得TPO cDNA。使用BM公司高保真的Taq系统共进行30次循环的PCR。反应条件为52℃退火40秒,72℃延伸55秒以及94℃变性20秒,生成EPO cDNA和TPO cDNA。它们分别被克隆到克隆载体pGEM-T(Promega公司)上。即,将PCR产物从1%琼脂糖凝胶中洗脱出来,并连接到pGEM-T上,然后导入到E.coli NM522中。将转化的E.coli在含有X-gal/IPTG的LB-氨苄青霉素平板上培养过夜。质粒从白色菌落中纯化并用限制性酶SacI和SacII处理,以便筛选含有各自cDNA的菌落。该步骤获得的载体命名为pGEM-EPO和pGEM-TPO,经测序后用于下列程序的模板。
采用BM公司高保真的Taq系统,以pGEM-TPO为模板,EL1和T2为引物(各50pmol),在反应条件为50℃退火40秒、72℃延伸45秒以及94℃变性20秒下,共进行30次循环的PCR,从而获得本发明中所用的TPO的CTP基因LTP。引物EL1含有来自限制性酶StuI识别位点的基因,该位点靠近EPO的3’端,同时含有LTP基因5’端的一部分。在1%琼脂糖凝胶中鉴别出约534bp的基因片段(LTP)。该基因编码TPO羧基端178个氨基酸(氨基酸位置176-353)(附图1)。
另一方面,采用pGEM-EPO为模板以及引物EP1和EP2进行PCR扩增,只产生EPO基因。
由此获得的EPO和LTP基因分别用限制性酶StuI处理。然后采用Qiagen抽提试剂盒纯化EPO和LTP基因的片段并用连接酶连接。以EPO和LTP基因的连接产物为模板,采用引物EP11和L2(各50pmol)和BM公司高保真的Taq系统在反应条件为55℃退火40秒、72℃延伸60秒以及94℃变性20秒下,共进行30次循环的PCR,生成所需的含有约1113bp的融合基因ELTP。将该基因以上述相同方式克隆到克隆载体pGEM-T中,然后测序(pGEM-ELTP,附图3a)。
通过合成和自身引导PCR程序获得STP基因。合成的DNA片段为ES1、S2、S3和L2。4种DNA片段各取1μl(50pmol/μl),采用BM公司高保真的Taq系统在反应条件为55℃退火40秒、72℃延伸40秒以及94℃变性20秒下,共进行15次循环的PCR。在1%琼脂糖凝胶上鉴定了为约50bp的基因片段(STP基因)。该基因编码TPO羧基端的17个氨基酸(氨基酸位置337-353)(附图1)。
以pGEM-EPO为模板,采用引物EP11和EP2以上述的相同方式进行PCR扩增,只生成EPO基因。将该EPO基因和STP基因同时用作模板,并以EP11和L2为引物,采用BM公司高保真的Taq系统在反应条件为58℃退火40秒、72℃延伸50秒以及94℃变性20秒下,共进行30次循环的PCR,最终生成所需的约630bp的融合基因ESTP基因。将该基因克隆到克隆载体pGEM-T上,并测序(pGEM-ESTP,附图3b)。
实施例2:表达载体pcDNA-ELTP和pcDNA-ESTP的构建
Invitrogen公司的pcDNA3.1载体用作表达载体。克隆到pGEM-T载体上的ELTP和ESTP基因分别在末端含有HindIII和BamHI识别位点。pcDNA3.1、pGEM-ELTP和pGEM-ESTP分别用限制性酶HindIII和BamHI处理。线性pcDNA3.1、ELTP和ESTP基因在琼脂糖凝胶上用Qiagen提取试剂盒分离。在pcDNA3.1与ELTP或ESTP连接后,将连接产物导入E.coli NM522中。将质粒从转化的E.coli在LB-氨苄青霉素平板上经培养过夜后所形成的菌落中分离出来,并用限制性酶HindIII和BamHI处理。然后含有ELTP或ESTP基因的菌落经1%琼脂糖凝胶电泳后被筛选出来。这些质粒分别命名为pcDNA-ELTP和pcDNA-ESTP(附图3)。
实施例3:CHO细胞的转化及表达
将CHO细胞(DG44)在60mm细胞培养皿中培养至40-80%汇合(1-4×105细胞/60mm平皿)。将3μl的superfection试剂(BM公司)和97μl的细胞培养基(带有基质的α-MEM、无血清、无抗体)混合均匀,然后其中加入质粒pcDNA-ELTP(=0.1μg/μl,约2μg)和具有dhfr基因的载体pLTRdhfr26(ATCC37295,0.2μg)。室温下混合物反应5-10分钟,然后加入如上所制备的细胞中。一天后,用含有G418的培养基(无基质的α-MEM,10%FBS)更新原培养基,含量为500μg/ml。然后用含有500μg/ml G418的培养基连续更新培养基7-10天,在此期间,无G418抗性基因的细胞和阴性对照细胞被完全杀死。将筛选出的细胞在G418培养基上充分培养,并用BM公司的EPO ELISA试剂盒鉴定所表达的ELTP蛋白。相同方法应用到pcDNA-ESTP。
实施例4:被表达融合蛋白的纯化
采用抗EPO单克隆抗体(R&D System公司)制备用于分离和纯化的亲和树脂,方法如下:
将0.3g CNBr活化的琼脂糖凝胶4B(Sepharose 4B)在1mM HCl中溶胀20分钟,然后将树脂转移至柱内,并用1mM HCl洗涤。用4ml偶联缓冲液(0.1M NaHCO3,0.5M NaCl,pH8.3)洗涤树脂,立即与包含在4ml偶联缓冲液中的抗EPO单克隆抗体(500μg/瓶)在管内混合,并室温下震荡试管反应2小时。用封闭缓冲液(0.2M甘氨酸,pH8.0)更新后,震荡试管使树脂在室温下反应2小时。然后,将树脂按序用6.5ml偶联缓冲液、6.5ml醋酸缓冲液(0.1M醋酸,0.5M NaCl,pH4)以及6.5ml偶联缓冲液洗涤。采用如此获得的树脂制备柱子,并按如下所述进行纯化。
将细胞在无血清培养基中培养一天,并采用Centriprep(Millipore,截留分子量10,000)将培养基浓缩约5倍。将该浓缩液以20ml/小时流速装载到预先用PBS平衡过的柱上,用PBS再次洗脱。将洗脱缓冲液(0.1M甘氨酸,pH2.8)施加到柱上,并将洗脱液立即用1M Tris滴定至pH7.5。纯化ELTP和ESTP的SDS-PAGE结果显示在附图4中。用SDS-PAGE和银染分析,纯度至少为97%。
实施例5:生物分析方法测定活性
将苯肼每天一次以60mg/kg的剂量注射到小鼠中,连续2天。3天后分离出膨大的脾脏并用均质机研磨,得到脾细胞。脾细胞稀释至6×106细胞/ml,然后将100μl细胞液转移入96孔板的每个孔中。将0-500mU/ml的EPO标准品和100mU/ml的表达融合蛋白加入到每个孔中,并让板在CO2培养箱中37℃放置22小时。每孔中加入50μl二甲基3[H]-胸苷(20μCi/ml),在相同培养箱中反应2小时,然后将每孔反应液吸附到玻璃滤纸(Nunc 1-73164)上。滤纸用生理盐水洗涤三次,然后用β计数器测定每个滤纸上放射量。融合蛋白、ELTP和ESTP的活性显示与EPO标准品活性相当或更高,这表明融合进EPO的羧基端不抑制EPO自身的活性。
实施例6:药代动力学实验
对小鼠进行药代动力学实验以测定所制备的候选物质是否真正延长了体内半寿期。将根据实施例5的方法纯化的融合蛋白以20单位/小鼠的量静脉施用给4只小鼠。为了鉴定血液中的定时浓度,每间隔30分钟从小鼠中取出血液,并采用宝灵曼(BM)公司的EIA试剂盒测定浓度。结果显示在附图5中。正如附图5所见,ETLP和ESLP分别比对照EPO的半寿期显示长约三倍(EPO的半寿期为22分钟,ELTP为60分钟,以及ESTP为57分钟)。
工业实用性
根据本发明的融合蛋白由于具有增加碳水化合物链的氨基酸,但又不影响EPO的固有活性,显著增加了EPO体内半寿期。进一步,由于融合肽、LTP或STP体内早已存在,因此当融合蛋白给人体施用时不会带来任何抗原性问题。
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<212>PRT
<213>人工序列
<220>
<223>红细胞生成素(EPO)与人血小板生成素的羧基端肽(STP)形
成的融合蛋白(ESTP)
<400>4
Met Gly Val His Glu Cys Pro Ala Trp Leu Trp Leu Leu Leu Ser Leu
1 5 10 15
Leu Ser Leu Pro Leu Gly Leu Pro Val Leu Gly Ala Pro Pro Arg Leu
20 25 30
Ile Cys Asp Ser Arg Val Leu Glu Arg Tyr Leu Leu Glu Ala Lys Glu
35 40 45
Ala Glu Asn Ile Thr Thr Gly Cys Ala Glu His Cys Ser Leu Asn Glu
50 55 60
Asn Ile Thr Val Pro Asp Thr Lys Val Asn Phe Tyr Ala Trp Lys Arg
65 70 75 80
Met Glu Val Gly Gln Gln Ala Val Glu Val Trp Gln Gly Leu Ala Leu
85 90 95
Leu Ser Glu Ala Val Leu Arg Gly Gln Ala Leu Leu Val Asn Ser Ser
100 105 110
Gln Pro Trp Glu Pro Leu Gln Leu His Val Asp Lys Ala Val Ser Gly
115 120 125
Leu Arg Ser Leu Thr Thr Leu Leu Arg Ala Leu Gly Ala Gln Lys Glu
130 135 140
Ala Ile Ser Pro Pro Asp Ala Ala Ser Ala Ala Pro Leu Arg Thr Ile
145 150 155 160
Thr Ala Asp Thr Phe Arg Lys Leu Phe Arg Val Tyr Ser Asn Phe Leu
165 170 175
Arg Gly Lys Leu Lys Leu Tyr Thr Gly Glu Ala Cys Arg Thr Gly Asp
180 185 190
Pro Leu Leu Asn Thr Ser Tyr Thr His Ser Gln Asn Leu Ser Gln Glu
195 200 205
Gly
<210>5
<211>29
<212>DNA
<213>人工序列
<220>
<223>具有与EPO cDNA末端序列互补的核苷酸序列的引物EP1
<400>5
atgggggcac gaatgtcctg cctggctgg 29
<210>6
<211>20
<212>DNA
<213>人工序列
<220>
<223>具有与EPO cDNA末端序列互补的核苷酸序列的引物EP2
<400>6
gtcccctgtc ctgcaggcct 20
<210>7
<211>24
<212>DNA
<213>人工序列
<220>
<223>具有与TPO cDNA末端序列互补的核苷酸序列的引物T1
<400>7
atggatctga ctgaattgct cctc 24
<210>8
<211>27
<212>DNA
<213>人工序列
<220>
<223>具有与TPO cDNA末端序列互补的核苷酸序列的引物T2
<400>8
ttacccttcc tgagacagat tctggga 27
<210>9
<211>43
<212>DNA
<213>人工序列
<220>
<223>用于PCR扩增以获得所需基因LTP的引物EL1
<400>9
gaggcctgca ggacagggga cgccccaccc accacagctg tcc 43
<210>10
<211>25
<212>DNA
<213>人工序列
<220>
<223>用于PCR扩增以获得所需融合基因ELTP和ESTP的引物EP11
<400>10
taagcttatg ggggtgcacg aatgt 25
<210>11
<211>29
<212>DNA
<213>人工序列
<220>
<223>用于PCR扩增以获得所需融合基因ELTP和ESTP的引物L2
<400>11
tggattctta cccttcctga gacagattc 29
<210>12
<211>35
<212>DNA
<213>人工序列
<220>
<223>用于PCR改组以获得所需基因STP的引物ES1
<400>12
aggggaggcc tgcaggacag gggaccctct tctaa 35
<210>13
<211>27
<212>DNA
<213>人工序列
<220>
<223>用于PCR改组以获得所需基因STP的引物S2
<400>13
gtgggtgtag gatgtgttta gaagagg 27
<210>14
<211>25
<212>DNA
<213>人工序列
<220>
<223>用于PCR改组以获得所需基因STP的引物S3
<400>14
tacacccact cccagaatct gtctc 25
Claims (5)
1.一种融合蛋白,其中将血小板生成素的羧基端肽与人红细胞生成素的羧基端融合,所述羧基端肽的C端为血小板生成素的第353位氨基酸,而其N端为血小板生成素的第176位至第337位氨基酸。
2.权利要求1所述的融合蛋白,其中羧基端肽为血小板生成素的第176-353位的氨基酸,其序列描述在SEQ ID No.1中。
3.权利要求1所述的融合蛋白,其中羧基端肽为血小板生成素的第337-353位的氨基酸,其序列描述在SEQ ID No.2中。
4.编码如权利要求1-3任一项所述融合蛋白的核酸。
5.一种制备具有增强了的人红细胞生成素体内活性的融合蛋白的方法,所述方法包括对用重组载体转化的宿主细胞系的培养,所述重组载体含有如权利要求4所述的核酸。
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
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| KR10-2001-0074975A KR100467750B1 (ko) | 2001-11-29 | 2001-11-29 | 생체내 에리스로포이에틴 활성이 증진된 융합단백질 |
| KR74975/2001 | 2001-11-29 |
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| CN1421461A CN1421461A (zh) | 2003-06-04 |
| CN100390201C true CN100390201C (zh) | 2008-05-28 |
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| CNB021301557A Expired - Fee Related CN100390201C (zh) | 2001-11-29 | 2002-08-23 | 具有增强红细胞生成素体内活性的融合蛋白 |
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| US (1) | US7098318B2 (zh) |
| EP (1) | EP1319712B1 (zh) |
| JP (1) | JP3860097B2 (zh) |
| KR (1) | KR100467750B1 (zh) |
| CN (1) | CN100390201C (zh) |
| AR (1) | AR036384A1 (zh) |
| AT (1) | ATE460483T1 (zh) |
| AU (1) | AU2002300359B2 (zh) |
| BR (1) | BRPI0203394B1 (zh) |
| CA (1) | CA2394572C (zh) |
| DE (2) | DE10235248B4 (zh) |
| ES (1) | ES2339426T3 (zh) |
| FR (1) | FR2832716B1 (zh) |
| GB (1) | GB2382580B (zh) |
| IT (1) | ITMI20021803A1 (zh) |
| MX (1) | MXPA02008131A (zh) |
| MY (1) | MY122935A (zh) |
| NZ (1) | NZ520442A (zh) |
| RU (1) | RU2225220C1 (zh) |
| SG (1) | SG117416A1 (zh) |
| TW (1) | TWI237056B (zh) |
| WO (1) | WO2003046013A1 (zh) |
| ZA (1) | ZA200206172B (zh) |
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| US7345019B1 (en) * | 1999-04-13 | 2008-03-18 | The Kenneth S. Warren Institute, Inc. | Modulation of excitable tissue function by peripherally administered erythropoietin |
| US7767643B2 (en) | 2000-12-29 | 2010-08-03 | The Kenneth S. Warren Institute, Inc. | Protection, restoration, and enhancement of erythropoietin-responsive cells, tissues and organs |
| US20030072737A1 (en) * | 2000-12-29 | 2003-04-17 | Michael Brines | Tissue protective cytokines for the protection, restoration, and enhancement of responsive cells, tissues and organs |
| CN1897959A (zh) * | 2003-09-29 | 2007-01-17 | 沃伦药品公司 | 用于治疗和预防脓毒病和粘连形成的组织保护细胞因子 |
| US7625564B2 (en) | 2006-01-27 | 2009-12-01 | Novagen Holding Corporation | Recombinant human EPO-Fc fusion proteins with prolonged half-life and enhanced erythropoietic activity in vivo |
| US8048849B2 (en) | 2006-02-03 | 2011-11-01 | Modigene, Inc. | Long-acting polypeptides and methods of producing same |
| US8946155B2 (en) | 2006-02-03 | 2015-02-03 | Opko Biologics Ltd. | Long-acting polypeptides and methods of producing and administering same |
| US9458444B2 (en) | 2006-02-03 | 2016-10-04 | Opko Biologics Ltd. | Long-acting coagulation factors and methods of producing same |
| US10351615B2 (en) | 2006-02-03 | 2019-07-16 | Opko Biologics Ltd. | Methods of treatment with long-acting growth hormone |
| US20150038413A1 (en) | 2006-02-03 | 2015-02-05 | Opko Biologics Ltd. | Long-acting polypeptides and methods of producing and administering same |
| US9249407B2 (en) | 2006-02-03 | 2016-02-02 | Opko Biologics Ltd. | Long-acting coagulation factors and methods of producing same |
| US20140113860A1 (en) | 2006-02-03 | 2014-04-24 | Prolor Biotech Ltd. | Long-acting polypeptides and methods of producing and administering same |
| US10221228B2 (en) | 2006-02-03 | 2019-03-05 | Opko Biologics Ltd. | Long-acting polypeptides and methods of producing and administering same |
| US7553941B2 (en) * | 2006-02-03 | 2009-06-30 | Modigene Inc | Long-acting polypeptides and methods of producing same |
| BRPI0814465B1 (pt) | 2007-07-26 | 2021-11-23 | Novagen Holding Corporation | Proteína de fusão, dímero, método para produzir uma proteína de fusão, linhagem de célula, usos de uma proteína de fusão e de uma composição farmacêutica e composição farmacêutica |
| CN101863982A (zh) * | 2009-04-17 | 2010-10-20 | 哈药集团生物工程有限公司 | 一种用于升高血小板的融合蛋白及其制备方法 |
| US9663778B2 (en) | 2009-07-09 | 2017-05-30 | OPKO Biologies Ltd. | Long-acting coagulation factors and methods of producing same |
| CN103864913A (zh) * | 2012-12-18 | 2014-06-18 | 联亚生技开发股份有限公司 | 重组蛋白 |
| WO2014159813A1 (en) | 2013-03-13 | 2014-10-02 | Moderna Therapeutics, Inc. | Long-lived polynucleotide molecules |
| US20150158926A1 (en) | 2013-10-21 | 2015-06-11 | Opko Biologics, Ltd. | Long-acting polypeptides and methods of producing and administering same |
| US10960058B2 (en) | 2015-06-19 | 2021-03-30 | Opko Biologics Ltd. | Long-acting coagulation factors and methods of producing same |
| CN118085104A (zh) | 2016-07-11 | 2024-05-28 | Opko生物科学有限公司 | 长效凝血因子及其制备方法 |
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- 2002-08-01 ES ES02016953T patent/ES2339426T3/es not_active Expired - Lifetime
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- 2002-08-01 AT AT02016953T patent/ATE460483T1/de active
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- 2002-08-06 GB GB0218252A patent/GB2382580B/en not_active Expired - Fee Related
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- 2002-08-23 CN CNB021301557A patent/CN100390201C/zh not_active Expired - Fee Related
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- 2002-08-30 RU RU2002123438/15A patent/RU2225220C1/ru not_active IP Right Cessation
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