Molecular characterization of three rat liver serine‐protease inhibitors affected by inflammation and hypophysectomy

Pagès, Gilles; Rouayrenc, J.F.; Cam, Ginette Le; Mariller, Marcel; Cam, Alphonse Le

doi:10.1111/j.1432-1033.1990.tb15587.x

Cited by 53 publications

(43 citation statements)

References 38 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…It has been shown that inflammation causes a decrease in the Spi 2 expression. 26 AdCTGF and AdTGF␤1 up-regulate Spi 2 RNA in mouse liver compared with the adenoviral control AdE1. Spi 2 is constitutively expressed in liver tissue of normal rats and significantly decreased during inflammation.…”

Section: Discussionmentioning

confidence: 92%

“…Spi 2 is constitutively expressed in liver tissue of normal rats and significantly decreased during inflammation. 26 The up-regulation of protease inhibitors is a common feature of overexpression of TGF␤1 and CTGF and may reflect the role that these genes play in fibrosis. 6,18 It has been shown that synthetic serine protease inhibitors, in combination with a metalloprotease 1 inhibitor, prevent the invasion and metastasis of tumor cells 27 by inhibiting the degradation of the extra-cellular matrix.…”

Section: Discussionmentioning

confidence: 99%

See 1 more Smart Citation

Profiling of genes which are differentially expressed in mouse liver in response to adenoviral vectors and delivered genes

2000

Gene Ther

View full text Add to dashboard Cite

Section: Discussionmentioning

confidence: 92%

Section: Discussionmentioning

confidence: 99%

Profiling of genes which are differentially expressed in mouse liver in response to adenoviral vectors and delivered genes

2000

Gene Ther

View full text Add to dashboard Cite

“…The procedure for run-on analysis, which includes incubation of the nuclei with [a-"PIUTP, purification of total cellular RNA and hybridization to templates immobilized on a nylon membrane (Hybond NC, Amersham) has been previously described [16]. The following plasmids were used as hybridization templates: pUC19 bearing 0.52 kb of the spi 2.1 cDNA 5' region [2]; pUC19 bearing the 0.35-kb 3' UTR specific extension of the spi 2.3 gene [2]; pBR322 harboring 0.65 kb of the rat a,-macroglobulin cDNA [17]; pBR322 bearing 1.6 kb of the mouse p-actin cDNA [18]; pBR322 containing 1.2 kb of the rat albumin cDNA [19]; Bluescript SK+ bearing 0.7 kb of the rat a,-acid glycoprotein cDNA [20]; pUC 19 bearing 1.25 kb of the rat insulin receptor tyrosine kinase inhibitor cDNA @p63) [21]. The amount of labeled transcripts newly synthetized by control and inflamed rat liver nuclei used for hybridization to templates corresponded to 20 X 1 O6 trichloroacetic-acid-precipitable counts.…”

Section: Materials [A-32p]datp (3000 Cdmmolmentioning

confidence: 99%

“…Nuclei isolated from the liver [15] of normal or turpentine inflamed rats [2] were used to evaluate the in vivo rates of transcription initiation. The procedure for run-on analysis, which includes incubation of the nuclei with [a-"PIUTP, purification of total cellular RNA and hybridization to templates immobilized on a nylon membrane (Hybond NC, Amersham) has been previously described [16].…”

Section: Materials [A-32p]datp (3000 Cdmmolmentioning

confidence: 99%

“…Site-specific mutations were introduced using asymmetric PCR [13]. The 348-bp extension specific of the spi 2.3 3' UTR region located at nucleotides 1712-2060 of the cDNA [2] or the three restriction fragments of 64, 125 and 159 bp generated by its cleavage with Pstl, or two elements of the coding spi 2.3 region (A, nucleotides 390-824; B, nucleotides 824-1020) were subcloned at various positions into CAT vectors. A pEMBL construct bearing the aldolase B promoter (nucleotides -190 to f14) [14] was kindly provided by M. Raymondjean (ICGM, Paris, France).…”

Section: Materials [A-32p]datp (3000 Cdmmolmentioning

confidence: 99%

See 1 more Smart Citation