ERK1/2 pathway involved in the expression of ETB receptors of the culturing smooth muscle cells of rat mesenteric artery

Luo, Guogang; Cao, Y X; Xu, Cang-Bao; Ma, A Q; Edvinsson, Lars

ERK1/2 pathway involved in the expression of ETB receptors of the culturing smooth muscle cells of rat mesenteric artery

Mark

Luo, Guogang ^LU ; Cao, Y X ; Xu, Cang-Bao ^LU ; Ma, A Q and Edvinsson, Lars ^LU (2006) In Yao Xue Xue Bao 41(3). p.257-262

Abstract: AIM: To determine the involvement of extracellular signal-regulated kinase 1/2 (ERK1/2) pathway in the expression of endothelin receptor type B (ETB) during culture.

METHODS: SB386023, a specific inhibitor for ERK1/2 pathway, was used to define the intracellular signaling pathway for the upregulation of ETB receptors and sarafotoxin 6c (S6c), a selective agonist for ETB receptors, induced contraction in isolated rat superior mesenteric arteries. The contraction was recorded by a sensitive in vitro myograph and the receptor mRNA was quantified by a real-time PCR. The phosphorylated ERK1/2 proteins were analyzed by phosphoELISA assay.

RESULTS: S6c induced strong contractile responses of the artery after culture for 24 h,... (More); AIM: To determine the involvement of extracellular signal-regulated kinase 1/2 (ERK1/2) pathway in the expression of endothelin receptor type B (ETB) during culture.

METHODS: SB386023, a specific inhibitor for ERK1/2 pathway, was used to define the intracellular signaling pathway for the upregulation of ETB receptors and sarafotoxin 6c (S6c), a selective agonist for ETB receptors, induced contraction in isolated rat superior mesenteric arteries. The contraction was recorded by a sensitive in vitro myograph and the receptor mRNA was quantified by a real-time PCR. The phosphorylated ERK1/2 proteins were analyzed by phosphoELISA assay.

RESULTS: S6c induced strong contractile responses of the artery after culture for 24 h, while there was no response to S6c in fresh vessel segments. The enhanced contractile response to S6c paralleled with an increase of mRNA for ETB receptors. The phosphorylated ERK1/2 proteins significantly increased after culture for 3 h. After co-culture with SB386023 for 24 h, S6c-induced contractions significantly decreased with reduction of Emax from (217 +/- 14) % to (127 +/- 23) % (P <0.01). This response paralleled with a decreased level of ETB receptor mRNA.

CONCLUSION: ERK1/2 pathway was involved in the up-regulation of ETB receptors on smooth muscle cells isolated from rat mesenteric arteries during culture. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/1137029

author

Luo, Guogang ^LU ; Cao, Y X ; Xu, Cang-Bao ^LU ; Ma, A Q and Edvinsson, Lars ^LU

organization

Medicine, Lund

publishing date

2006

type

Contribution to journal

publication status

published

subject

Other Clinical Medicine

in

Yao Xue Xue Bao

volume

41

issue

3

pages

257 - 262

publisher

Chinese Electronic Periodical Services

external identifiers

scopus:33646442464

ISSN

0513-4870

language

English

LU publication?

yes

id

83998e61-01c9-426b-8ec0-17f9446c753b (old id 1137029)

date added to LUP

2016-04-01 17:04:05

date last changed

2024-01-11 20:02:05

@article{83998e61-01c9-426b-8ec0-17f9446c753b,
  abstract     = {{AIM: To determine the involvement of extracellular signal-regulated kinase 1/2 (ERK1/2) pathway in the expression of endothelin receptor type B (ETB) during culture.<br/><br>
METHODS: SB386023, a specific inhibitor for ERK1/2 pathway, was used to define the intracellular signaling pathway for the upregulation of ETB receptors and sarafotoxin 6c (S6c), a selective agonist for ETB receptors, induced contraction in isolated rat superior mesenteric arteries. The contraction was recorded by a sensitive in vitro myograph and the receptor mRNA was quantified by a real-time PCR. The phosphorylated ERK1/2 proteins were analyzed by phosphoELISA assay.<br/><br>
RESULTS: S6c induced strong contractile responses of the artery after culture for 24 h, while there was no response to S6c in fresh vessel segments. The enhanced contractile response to S6c paralleled with an increase of mRNA for ETB receptors. The phosphorylated ERK1/2 proteins significantly increased after culture for 3 h. After co-culture with SB386023 for 24 h, S6c-induced contractions significantly decreased with reduction of Emax from (217 +/- 14) % to (127 +/- 23) % (P &lt;0.01). This response paralleled with a decreased level of ETB receptor mRNA.<br/><br>
CONCLUSION: ERK1/2 pathway was involved in the up-regulation of ETB receptors on smooth muscle cells isolated from rat mesenteric arteries during culture.}},
  author       = {{Luo, Guogang and Cao, Y X and Xu, Cang-Bao and Ma, A Q and Edvinsson, Lars}},
  issn         = {{0513-4870}},
  language     = {{eng}},
  number       = {{3}},
  pages        = {{257--262}},
  publisher    = {{Chinese Electronic Periodical Services}},
  series       = {{Yao Xue Xue Bao}},
  title        = {{ERK1/2 pathway involved in the expression of ETB receptors of the culturing smooth muscle cells of rat mesenteric artery}},
  volume       = {{41}},
  year         = {{2006}},
}

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ERK1/2 pathway involved in the expression of ETB receptors of the culturing smooth muscle cells of rat mesenteric artery