Laser capture microdissection and real-time PCR for analysis of glomerular endothelin-1 gene expression in mesangiolysis of rat anti-Thy 1.1 and murine Habu Snake Venom glomerulonephritis

A Dimmler; C S Haas; S Cho; M Hattler; C Forster; H Peters; H O Schöcklmann; K Amann

doi:10.1097/00019606-200306000-00007

Laser capture microdissection and real-time PCR for analysis of glomerular endothelin-1 gene expression in mesangiolysis of rat anti-Thy 1.1 and murine Habu Snake Venom glomerulonephritis

Diagn Mol Pathol. 2003 Jun;12(2):108-17. doi: 10.1097/00019606-200306000-00007.

Authors

A Dimmler¹, C S Haas, S Cho, M Hattler, C Forster, H Peters, H O Schöcklmann, K Amann

Affiliation

¹ Department of Pathology, University of Erlangen-Nürnberg, Germany.

PMID: 12766616
DOI: 10.1097/00019606-200306000-00007

Abstract

Molecular analysis of pathologic changes in glomeruli requires methods allowing rapid and exact detection of alterations in gene expression. Here, we analyzed endothelin-1 (ET-1) mRNA expression in mesangiolytic glomeruli during the course of a rat and murine model of mesangioproliferative glomerulonephritis (GN). A novel method combining laser capture microdissection (LCM), which permits the precise removal of selected mesangiolytic glomeruli, with a highly sensitive real-time RT-PCR technique was used. Anti-Thy 1.1. GN was introduced in male Sprague-Dawley rats (1.0 mg/kg body weight of OX-7 IV) and Habu Snake Venom GN was introduced in C57BL6 mice (habu snake venom toxin 6 mg/kg body weight IV). The degree of mesangiolysis during both GNs was analyzed using a semiquantitative scoring system. Mesangiolytic glomeruli were microdissected at different days of the diseases (day 2, 6, and 12 in anti-Thy 1.1 GN and days 1, 3, 7, and 14 in Habu Snake Venom GN) and from normal control animals. After RNA extraction and cDNA synthesis, ET-1 gene expression was measured by real-time RT-PCR. In parallel, in anti-Thy 1.1. GN ET-1 mRNA expression was analyzed using semiquantitative nonradioactive in situ hybridization; ET-1 protein expression was investigated by immunohistochemistry. Mesangiolysis peaked at day 6 in anti-Thy1.1 GN and at day 1 in Habu Snake Venom GN. Mesangiolytic glomeruli were easily microdissected on cryostat sections in both models; quantification of mRNA with RT-PCR was reliable and reproducible. Glomerular ET-1 mRNA expression increased during the course of anti-Thy 1.1 GN and Habu Snake Venom GN peaked when mesangiolysis was most pronounced. This was seen by RT-PCR after glomerular LCM and by in situ hybridization; in parallel, glomerular ET-1 protein expression was increased. Combination of LCM and RT-PCR is a reliable method for quantification of localized gene expression in isolated renal structures. The above data argue for an important role of ET-1 in pathogenesis and/or repair of mesangiolysis in experimental mesangioproliferative GN.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Antibodies, Monoclonal / pharmacology
Crotalid Venoms / toxicity
Disease Models, Animal
Endothelin-1 / genetics*
Endothelin-1 / metabolism
Gene Expression*
Glomerular Mesangium / drug effects
Glomerular Mesangium / metabolism
Glomerular Mesangium / pathology*
Glomerulonephritis, Membranoproliferative / etiology
Glomerulonephritis, Membranoproliferative / metabolism
Glomerulonephritis, Membranoproliferative / pathology*
Laser Therapy
Male
Mice
Mice, Inbred C57BL
Microdissection / methods*
RNA, Messenger / metabolism
Rats
Rats, Sprague-Dawley
Reverse Transcriptase Polymerase Chain Reaction*
Thy-1 Antigens / immunology

Substances

Antibodies, Monoclonal
Crotalid Venoms
Endothelin-1
RNA, Messenger
Thy-1 Antigens