重组AAV-2/人凝血因子IX(Vector Gene Technology)(rAAV-2-hFIX) - 药物靶点：factor IX_专利_临床

概要

基本信息

药物类型

腺相关病毒基因治疗

别名-

靶点

factor IX

作用机制

凝血因子IX基因转移

治疗领域

遗传病与畸形血液及淋巴系统疾病其他疾病

在研适应症-

非在研适应症

血友病B

原研机构

本元正阳基因技术有限公司

在研机构-

非在研机构

本元正阳基因技术有限公司

最高研发阶段无进展临床1期

首次获批日期-

最高研发阶段(中国)无进展

特殊审评-

登录后查看时间轴

关联

100 项与重组AAV-2/人凝血因子IX(Vector Gene Technology) 相关的临床结果

登录后查看更多信息

100 项与重组AAV-2/人凝血因子IX(Vector Gene Technology) 相关的转化医学

登录后查看更多信息

100 项与重组AAV-2/人凝血因子IX(Vector Gene Technology) 相关的专利（医药）

登录后查看更多信息

3

项与重组AAV-2/人凝血因子IX(Vector Gene Technology) 相关的文献（医药）

2005-09-01·Zhonghua xue ye xue za zhi = Zhonghua xueyexue zazhi

[Expression of coagulation factor IX in human CD34 + hematopoietic stem cells by adeno-associated virus 2].

Article

作者: Chen, Fang-ping ; Chen, Yan ; Wang, Guang-ping ; Peng, Jian-qiang ; Xin, Hong-ya ; Jian, Zai-fu ; Wu, Xin-hua ; Wu, Xiao-bing

OBJECTIVE:

To investigate the expression of human coagulation factor IX (hFIX) gene in human umbilical cord blood (CB) CD34+ cells which was transfected with recombinant adeno-associated virus 2 (rAAV-2).

METHOD:

The CD34+ cells were transfected with rAAV-2/hFIX and cultured for 21 days for inducing differentiation into myeloid, erythroid and megakaryocytes, respectively. The expression of hFIX was studied at mRNA, protein and biological activity levels. The cytotoxicity of rAAV-2 to CD34+ cells was evaluated by cell proliferation, cell vitality, CD antigen expressions and CFU yields.

RESULTS:

The hFIX mRNA was expressed in the cultured cells which was verified by RT-PCR and DNA sequencing. An elevated level of hFIX expression and biological activities were detected with a maximum amount of 14.10 ng/10(6) cell x 24 h. During the period of 21 day culture, the cell vitality, cell proliferation, CD antigen expression and CFU yields between the transfected and un-transfected groups had no difference(P > 0.05).

CONCLUSION:

The human CB CD34+ cells are able to produce functional hFIX after transduction by rAAV-2/hFIX. The cell proliferation and differentiation capacities of the host CD34+ cells were not affected by rAAV-2.

2004-09-01·Zhonghua xue ye xue za zhi = Zhonghua xueyexue zazhi

[Preparation of rAAV2/hFIX and experimentally application to gene therapy for hemophilia B].

Article

作者: Peng, Ming ; Dong, Xiao-yan ; Yuan, Hong ; Peng, Jian-qiang ; Chen, Fang-ping ; Tan, Shu-ping ; Wu, Xiao-bing ; Chen, Li ; Xue, Jing-lun

OBJECTIVE:

To prepare the rAAV2/hFIX and evaluate the efficiency of the preparation on gene therapy of hemophilia B model mice.

METHODS:

The rAAV-2/hFIX was prepared by "one helper virus-one vector cell line" strategy and transfected both BHK-21 and C2C12 cells in vitro. The hFIX antigen level in cell culture supernatant was assayed. The rAAV-2/hFIX was injected into muscles of hemophilia B model mice and assayed the serum hFIX levels, hFIX clotting activity, bleeding time, 5 min bleeding volume.

RESULTS:

The hFIX antigen could be detected from 24 h till 120 h after BHK-21 and C2C12 cells were transfected with highest levels at 24 h reaching (51.0 +/- 6.5) ng/10(5) cells and (68.0 +/- 7.2) ng/10(5) cells, respectively. The rAAV2/hFIX injected mice could efficiently express hFIX and peaked at three weeks after injection, then slowly decreased but low level hFIX antigen was still detectable till 10 weeks after injection. There were significant differences between the high, middle and low dose groups of rAAV2/hFIX and the control group (P < 0.01), the plasma FIX clotting activities in the model mice were improved remarkably, bleeding time was greatly shortened and bleeding in 5 min was decreased. The hFIX expression level and FIX clotting activity of the high dose of rAAV2/hFIX group (1.6 x 10(13) v.g./kg) reached about (387.0 +/- 12.5) ng/ml plasma in contrast with the normal levels of (30.0 +/- 5.5)% at the third week after injection. No rAAV2 vector DNA was detected in the organs except for injected muscle tissue.

CONCLUSION:

The rAAV2/hFIX transfected BHK-21 and C2C12 cells could efficiently express hFIX antigen and was of therapeutic effects for the hemophilia B model mice by intramuscularly injection.The results provide the basis for clinical trial of rAAV2 gene therapy for hemophilia B.

2003-09-01·Yao xue xue bao = Acta pharmaceutica Sinica

[Quality control of recombinant adeno-associated virus type 2/human blood coagulation factor IX].

Article

作者: Wang, Jun-zhi ; Rao, Chun-ming ; Gao, Kai ; Wu, Xiao-bing

AIM:

To establish quality control requirements and methods for recombinant adeno-associated virus(rAAV) type 2/human blood coagulation factor IX (rAAV-2/hFIX).

METHODS:

Identification of rAAV genome fragments, potential contaminants including wild type AAV(wtAAV) and helper virus, were detected by PCR. Purity of rAAV-2/hFIX was analyzed by cation-exchange HPLC and SDS-PAGE. Virus partical numbers were performed by dot blot assay. hFIX expression was demonstrated by ELISA and potency of hFIX was verified by APTT.

RESULTS:

Identity of rAAV-2/hFIX was proved. Residues of wtAAV and helper virus were conformed to requirements. Purity of rAAV-2/hFIX were more than 98%. Partical numbers of rAAV-2/hFIX were more than 1.0 x 10(15) VG.L-1. hFIX expression was more than 20.0 micrograms.L-1. hFIX potency was verified by APTT following rAAV-2/hFIX injected to FIX gene knockout mice, potency results conformed to requirements.

CONCLUSION:

The methods and requirements had been established for quality control of rAAV-2/hFIX.

100 项与重组AAV-2/人凝血因子IX(Vector Gene Technology) 相关的药物交易

登录后查看更多信息