GENE-TRANSFER INTO THE RAT RENAL GLOMERULUS VIA A MESANGIAL CELL VECTOR - SITE-SPECIFIC DELIVERY, IN-SITU AMPLIFICATION, AND SUSTAINED EXPRESSION OF AN EXOGENOUS GENE IN-VIVO

被引：138

作者：

KITAMURA, M

TAYLOR, S

UNWIN, R

BURTON, S

SHIMIZU, F

FINE, LG

机构：

[1] UNIV LONDON UNIV COLL,SCH MED,INST UROL & NEPHROL,LONDON WC1E 6JJ,ENGLAND

[2] NIIGATA UNIV,SCH MED,INST NEPHROL,DEPT IMMUNOL,NIIGATA 951,JAPAN

来源：

JOURNAL OF CLINICAL INVESTIGATION | 1994年 / 94卷 / 02期

关键词：

GENETIC ENGINEERING; RETROVIRUS; BETA-GALACTOSIDASE; CELL TRANSPLANTATION; GENE THERAPY;

D O I：

10.1172/JCI117361

中图分类号：

R-3 [医学研究方法]; R3 [基础医学];

学科分类号：

1001 ;

摘要：

To evaluate the pathophysiological function of specific molecules in the renal glomerulus, selective, sustained, and modifiable expression of such molecules will be required. Towards achieving this end, we devised a gene transfer system using the glomerular mesangial cell as a vector for gene delivery. A reporter gene which encodes bacterial beta-galactosidase was introduced into cultured rat mesangial cells, and the stable transfectants were transferred into the fat kidney via the renal artery, leading to selective entrapment within the glomeruli. In the normal kidney, the reporter cells populated into 57 +/- 13% of glomeruli site specifically, and the expression of beta-galactosidase was sustained for 4 wk and declined thereafter. Within the glomerulus, some of the reporter cells remained in the glomerular capillaries, while others repopulated the mesangial area and, in part, extended their cytoplasmic processes toward the surrounding capillaries. When the cells were transferred into glomeruli subjected to transient mesangiolysis induced by monoclonal antibody 1-22-3, in situ expression of beta-galactosidase was amplified 7-12-fold, and the enhanced level of expression continued for up to 8 wk. The mesangial cell vector system thus achieves site-specific delivery of an exogenous gene into the glomerulus and is amenable to in situ amplification and sustained expression by preconditioning of the target site.

引用

页码：497 / 505

页数：9

共 29 条

[1] INTRAARTICULAR EXPRESSION OF BIOLOGICALLY-ACTIVE INTERLEUKIN-1 RECEPTOR-ANTAGONIST PROTEIN BY EX-VIVO GENE-TRANSFER
BANDARA, G
MUELLER, GM
GALEALAURI, J
TINDAL, MH
GEORGESCU, HI
SUCHANEK, MK
HUNG, GL
GLORIOSO, JC
ROBBINS, PD
EVANS, CH
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1993, 90 (22) : 10764 - 10768
[2] PROTEOLYTIC-ENZYMES AS MEDIATORS OF GLOMERULAR INJURY
BARICOS, WH
SHAH, SV
[J]. KIDNEY INTERNATIONAL, 1991, 40 (02) : 161 - 173
[3] BOSCH RJ, 1993, EXP NEPHROL, V1, P49
[4] BRADFORD MM, 1976, ANAL BIOCHEM, V72, P248, DOI 10.1016/0003-2697(76)90527-3
[5] CATTELL WR, 1989, CLIN RENAL IMAGING, pCH5
[6] CEPKO C, 1989, METHODS NEUROSCI, V1, P367
[7] CHOMCZYNSKI P, 1987, ANAL BIOCHEM, V162, P156, DOI 10.1016/0003-2697(87)90021-2
[8] A MODEL SYSTEM FOR INVIVO GENE-TRANSFER INTO THE CENTRAL-NERVOUS-SYSTEM USING AN ADENOVIRAL VECTOR
DAVIDSON, BL
ALLEN, ED
KOZARSKY, KF
WILSON, JM
ROESSLER, BJ
[J]. NATURE GENETICS, 1993, 3 (03) : 219 - 223
[9] INFUSION OF PLATELET-DERIVED GROWTH-FACTOR OR BASIC FIBROBLAST GROWTH-FACTOR INDUCES SELECTIVE GLOMERULAR MESANGIAL CELL-PROLIFERATION AND MATRIX ACCUMULATION IN RATS
FLOEGE, J
ENG, E
YOUNG, BA
ALPERS, CE
BARRETT, TB
BOWENPOPE, DF
JOHNSON, RJ
[J]. JOURNAL OF CLINICAL INVESTIGATION, 1993, 92 (06) : 2952 - 2962
[10] USE OF SINGLE VOIDED URINE SAMPLES TO ESTIMATE QUANTITATIVE PROTEINURIA
GINSBERG, JM
CHANG, BS
MATARESE, RA
GARELLA, S
[J]. NEW ENGLAND JOURNAL OF MEDICINE, 1983, 309 (25) : 1543 - 1546

← 1 2 3 →