Coupling of GnRH Concentration and the GnRH Receptor-Activated Gene Program

Yuen, Tony; Wurmbach, Elisa; Ebersole, Barbara J.; Ruf, Frederique; Pfeffer, Robert; Sealfon, Stuart C.

doi:10.1210/mend.16.6.0853

Cited by 59 publications

(34 citation statements)

References 23 publications

(29 reference statements)

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“…Egr-1 and Fra-1), the FC in response to insulin treatment was lower using the GeneChips® compared with real-time RT-PCR. This behavior is, however, not unusual and has been previously observed, especially for transcripts that are highly regulated (28,29). Among the 12 genes (including MCP-1) tested and validated using real-time RT-PCR, PAI-1 was the only gene that was classified differently by RT-PCR analysis (i.e.…”

Section: Table I Tnf-␣ Induces Changes Mimicking Metabolic Insulinsupporting

confidence: 66%

Expression Profiling Identifies Genes That Continue to Respond to Insulin in Adipocytes Made Insulin-resistant by Treatment with Tumor Necrosis Factor-α

Sartipy

Loskutoff

2003

Journal of Biological Chemistry

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We have employed microarray technology using RNA from normal 3T3-L1 adipocytes and from 3T3-L1 adipocytes made insulin-resistant by treatment with tumor necrosis factor-␣ to identify a new class of insulin-responsive genes. These genes continued to respond normally to insulin even though the adipocytes themselves were metabolically insulin-resistant, i.e. they displayed a significantly decreased rate of insulin-stimulated glucose uptake. Approximately 12,000 genes/expressed sequence tags (ESTs) were screened. Of these, 40 genes/ ESTs were identified that became insulin-resistant as expected (e.g. Socs-3, junB, and matrix metalloproteinase-11). However, 61 genes/ESTs continued to respond normally to insulin. Although some of these genes were previously shown to be regulated by insulin (e.g. Glut-1 and ␤ 3 -adrenergic receptor), other novel insulin-sensitive genes were also identified (e.g. Egr-1, epiregulin, Fra-1, and ABCA1). Real-time reverse transcription-PCR analysis confirmed the expression patterns of several of the differentially expressed genes. One gene that remained insulin-sensitive in the insulin-resistant adipocytes is the transcription factor Egr-1. Using an antisense strategy, we show that tissue factor and macrophage colony-stimulating factor, two cardiovascular risk factors, are downstream EGR-1 target genes in the adipocyte. Taken together, these data support the hypothesis that some signaling pathways remain insulin-sensitive in metabolically insulin-resistant adipocytes. These pathways may promote abnormal gene expression in hyperinsulinemic states like obesity and type II diabetes and thus may contribute to pathologies associated with these conditions.

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Section: Table I Tnf-␣ Induces Changes Mimicking Metabolic Insulinsupporting

confidence: 66%

Expression Profiling Identifies Genes That Continue to Respond to Insulin in Adipocytes Made Insulin-resistant by Treatment with Tumor Necrosis Factor-α

Sartipy

Loskutoff

2003

Journal of Biological Chemistry

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“…The present study also found higher expression of CYP6Z1 in the RSP strain, but the 1.31-fold overexpression was below our previously defined cutoff value of 1.5-fold. This result may be partially explained by the well known underestimation of gene expression ratios by microarrays compared with quantitative RT-PCR experiments (21). The present study also revealed a strong and significant overexpression of the gene CYP325A3 (1.72-fold).…”

Section: Genes Differentially Expressed In the Permethrin-resistant Ssupporting

confidence: 46%

The Anopheles gambiae detoxification chip: A highly specific microarray to study metabolic-based insecticide resistance in malaria vectors

David

Strode

Vontas

et al. 2005

Proc. Natl. Acad. Sci. U.S.A.

293

315

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Metabolic pathways play an important role in insecticide resistance, but the full spectra of the genes involved in resistance has not been established. We constructed a microarray containing unique fragments from 230 Anopheles gambiae genes putatively involved in insecticide metabolism [cytochrome P450s (P450s), GSTs, and carboxylesterases and redox genes, partners of the P450 oxidative metabolic complex, and various controls]. We used this detox chip to monitor the expression of the detoxifying genes in insecticide resistant and susceptible An. gambiae laboratory strains. Five genes were strongly up-regulated in the dichlorodiphenyltrichloroethane-resistant strain ZAN͞U. These genes included the GST GSTE2, which has previously been implicated in dichlorodiphenyltrichloroethane resistance, two P450s, and two peroxidase genes. GSTE2 was also elevated in the pyrethroidresistant RSP strain. In addition, the P450 CYP325A3, belonging to a class not previously associated with insecticide resistance, was expressed at statistically higher levels in this strain. The applications of this detox chip and its potential contribution to malaria vector insecticide resistance management programs are discussed.mosquito ͉ cytochrome P450 ͉ GST ͉ carboxylesterase

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“…This is likely due to the use of a pool of all the tumors as the common reference for this analysis, which might explain the only slight upregulation in individual tumors relative to the reference. The ability of the rtq-PCR to detect a difference between samples with or without FLJ14299 amplification is probably due to the wider dynamic range of this method (Yuen et al, 2002). C8orf2 and particularly BRF2, both mapping to the minimal region of amplification, showed the highest levels of overexpression in the microarray experiments and showed significant differences in expression when comparing amplified and nonamplified samples.…”

Section: Discussionmentioning

confidence: 99%

A 1 Mb minimal amplicon at 8p11–12 in breast cancer identifies new candidate oncogenes

et al. 2005

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Amplification of 8p11-12 is a well-known alteration in human breast cancers but the driving oncogene has not been identified. We have developed a high-resolution comparative genomic hybridization array covering 8p11-12 and analysed 33 primary breast tumors, 20 primary ovarian tumors and 27 breast cancer cell lines. Expression analysis of the genes in the region was carried out by using real-time quantitative PCR and/or oligo-microarray profiling. In all, 24% (8/33) of the breast tumors, 5% (1/20) of the ovary tumors and 15% (4/27) of the cell lines showed 8p11-12 amplification. We identified a 1 Mb segment of common amplification that excludes previously proposed candidate genes. Some of the amplified genes did not show overexpression, whereas for others, overexpression was not specifically attributable to amplification. The genes FLJ14299, C8orf2, BRF2 and RAB11FIP, map within the 8p11-12 minimal amplicon, two have a putative function consistent with an oncogenic role, these four genes showed a strong correlation between amplification and overexpression and are therefore the best candidate driver oncogenes at 8p12.

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Coupling of GnRH Concentration and the GnRH Receptor-Activated Gene Program

Cited by 59 publications

References 23 publications

Expression Profiling Identifies Genes That Continue to Respond to Insulin in Adipocytes Made Insulin-resistant by Treatment with Tumor Necrosis Factor-α

Expression Profiling Identifies Genes That Continue to Respond to Insulin in Adipocytes Made Insulin-resistant by Treatment with Tumor Necrosis Factor-α

The Anopheles gambiae detoxification chip: A highly specific microarray to study metabolic-based insecticide resistance in malaria vectors

A 1 Mb minimal amplicon at 8p11–12 in breast cancer identifies new candidate oncogenes

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