P Hwu scite author profile

P Hwu

3Publications

52Citation Statements Received

139Citation Statements Given

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133

Affiliations

Children's Hospital of Los Angeles

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Adenoviral Overexpression and Small Interfering RNA Suppression Demonstrate That Plasminogen Activator Inhibitor-1 Produces Elevated Collagen Accumulation in Normal and Keloid Fibroblasts

Tuan

Hwu

et al. 2008

The American Journal of Pathology

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Keloids are tumor-like skin scars that grow as a result of the aberrant healing of skin injuries, with no effective treatment. We provide new evidence that both overexpression of plasminogen activator inhibitor-1 (PAI-1) and elevated collagen accumulation are intrinsic features of keloid fibroblasts and that these characteristics are causally linked. Using seven strains each of early passage normal and keloid fibroblasts, the keloid strains exhibited inherently elevated collagen accumulation and PAI-1 expression in serumfree, 0.1% ITS؉ culture; larger increases in these parameters occurred when cells were cultured in 3% serum. To demonstrate a causal relationship between PAI-1 overexpression and collagen accumulation, normal fibroblasts were infected with PAI-1-expressing adenovirus. Such cells exhibited a two-to fourfold increase in the accumulation of newly synthesized collagen in a viral dose-dependent fashion in both monolayers and fibrin gel, provisional matrix-like cultures. Three different PAI-1-targeted small interfering RNAs, alone or in combination, produced greater than an 80% PAI-1 knockdown and reduced collagen accumulation in PAI-1-overexpressing normal or keloid fibroblasts. A vitronectin-binding mutant of PAI-1 was equipotent with wild-type PAI-1 in inducing collagen accumulation, whereas a complete protease inhibitor mutant retained approximately 50% activity. Thus, PAI-1 may use more than its protease inhibitory activity to control keloid collagen accumulation. PAI-1-targeted interventions , such as small interfering RNA and lentiviral short hairpin RNA-containing microRNA sequence suppression reported here , may have therapeutic utility in the prevention of keloid scarring.

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Posttranscriptional control of human gamma interferon gene expression in transfected mouse fibroblasts.

Young¹,

Varesio²,

Hwu³

1986

Mol. Cell. Biol.

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Human gamma interferon genomic DNA was introduced into NIH 3T3 fibroblasts by calcium phosphate precipitation and was not expressed in these cells at the cytoplasmic mRNA or protein level. Treatment of the transfected cells with cycloheximide (1 ,ug/ml) induced the accumulation of cytoplasmic gamma interferon mRNA and biologically active human gamma interferon. Analysis of the nuclear enriched RNA from untreated cells indicated that human gamma interferon mRNA was present, suggesting that cycloheximide may act by inhibiting a specific nuclease or may enhance the processing or transport of the RNA from the nucleus to the cytoplasm.Gamma interferon (IFN-y) is a unique lymphokine which has been reported to have a large number of immunoregulatory functions (for a recent review, see reference 26). Synthesis of this lymphokine appears to be limited to relatively few -cell types, namely T cells and large granular lymphocytes (LGL) (5, 25). Workers in this laboratory have analyzed the expression of the transfected human IFN-y genomic DNA in both a mouse T cell line and NIH 3T3 fibroblasts. It has been found that human IFN-y can be efficiently produced in mouse T cells but is not expressed in transfected mouse fibroblasts at the cytoplasmic RNA or protein level

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Posttranscriptional Control of Human Gamma Interferon Gene Expression in Transfected Mouse Fibroblasts

Young¹,

Varesio²,

Hwu³

1986

Molecular and Cellular Biology

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P Hwu

Adenoviral Overexpression and Small Interfering RNA Suppression Demonstrate That Plasminogen Activator Inhibitor-1 Produces Elevated Collagen Accumulation in Normal and Keloid Fibroblasts

Posttranscriptional control of human gamma interferon gene expression in transfected mouse fibroblasts.

Posttranscriptional Control of Human Gamma Interferon Gene Expression in Transfected Mouse Fibroblasts

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