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AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction

OBJECTIVE: Urinary bladder smooth muscle (UBSM) displays spontaneous action potentials and this potential is related to the phasic nature of spontaneous contractions in this tissue. The amplitude of a phasic contraction depends on the increase in Ca(2+) entry caused by membrane depolarization. Ryano...

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Autores principales: Boopathi, Ettickan, Javed, Elham, Addya, Shankar, Fortina, Paolo, Zderic, Stephen, Wein, Alan, Chacko, Samuel
Formato: Online Artículo Texto
Lenguaje:English
Publicado: AME Publishing Company 2016
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5143274/
http://dx.doi.org/10.21037/tau.2016.s283
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author Boopathi, Ettickan
Javed, Elham
Addya, Shankar
Fortina, Paolo
Zderic, Stephen
Wein, Alan
Chacko, Samuel
author_facet Boopathi, Ettickan
Javed, Elham
Addya, Shankar
Fortina, Paolo
Zderic, Stephen
Wein, Alan
Chacko, Samuel
author_sort Boopathi, Ettickan
collection PubMed
description OBJECTIVE: Urinary bladder smooth muscle (UBSM) displays spontaneous action potentials and this potential is related to the phasic nature of spontaneous contractions in this tissue. The amplitude of a phasic contraction depends on the increase in Ca(2+) entry caused by membrane depolarization. Ryanodine receptors (RyRs) in UBSM decreases the force production by decreasing the frequency of phasic contractions through interactions with large-conductance Ca(2+)-activated K(+) (BK) and small-conductance Ca(2+)-activated K(+) (SK) channels. Microarray and network analysis were employed to determine the changes in mRNA in 14-day obstructed murine bladders. We found that obstruction significantly down-regulated the RyRs in bladder smooth muscle (BSM). METHODS: Male C57Bl/6 mice were surgically obstructed and kept for 14 days. Sham-operated mice served as a control. Bladders were excised; urothelium scraped off with a scalpel, and the serosa was removed. BSM obtained from PBOO and sham control animals were used for microarray and western blotting RESULTS: Pathway-based analysis of these gene signatures showed significant number of under-expressed genes in obstructed bladder and they were mapped to proteins involved in calcium signaling. We focused our work on RyR protein expression in BSM. There was a four-fold reduction of RyR3 in BSM in 14-day obstructed groups as shown by microarray and immunoblotting compared to that of sham-operated animals. CONCLUSIONS: These results confirm that the RyR gene expression is down-regulated in obstructed murine bladder smooth muscle. FUNDING SOURCE(S): None
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spelling pubmed-51432742016-12-19 AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction Boopathi, Ettickan Javed, Elham Addya, Shankar Fortina, Paolo Zderic, Stephen Wein, Alan Chacko, Samuel Transl Androl Urol Abstract OBJECTIVE: Urinary bladder smooth muscle (UBSM) displays spontaneous action potentials and this potential is related to the phasic nature of spontaneous contractions in this tissue. The amplitude of a phasic contraction depends on the increase in Ca(2+) entry caused by membrane depolarization. Ryanodine receptors (RyRs) in UBSM decreases the force production by decreasing the frequency of phasic contractions through interactions with large-conductance Ca(2+)-activated K(+) (BK) and small-conductance Ca(2+)-activated K(+) (SK) channels. Microarray and network analysis were employed to determine the changes in mRNA in 14-day obstructed murine bladders. We found that obstruction significantly down-regulated the RyRs in bladder smooth muscle (BSM). METHODS: Male C57Bl/6 mice were surgically obstructed and kept for 14 days. Sham-operated mice served as a control. Bladders were excised; urothelium scraped off with a scalpel, and the serosa was removed. BSM obtained from PBOO and sham control animals were used for microarray and western blotting RESULTS: Pathway-based analysis of these gene signatures showed significant number of under-expressed genes in obstructed bladder and they were mapped to proteins involved in calcium signaling. We focused our work on RyR protein expression in BSM. There was a four-fold reduction of RyR3 in BSM in 14-day obstructed groups as shown by microarray and immunoblotting compared to that of sham-operated animals. CONCLUSIONS: These results confirm that the RyR gene expression is down-regulated in obstructed murine bladder smooth muscle. FUNDING SOURCE(S): None AME Publishing Company 2016-12 /pmc/articles/PMC5143274/ http://dx.doi.org/10.21037/tau.2016.s283 Text en 2016 Translational Andrology and Urology. All rights reserved.
spellingShingle Abstract
Boopathi, Ettickan
Javed, Elham
Addya, Shankar
Fortina, Paolo
Zderic, Stephen
Wein, Alan
Chacko, Samuel
AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
title AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
title_full AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
title_fullStr AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
title_full_unstemmed AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
title_short AB283. SPR-10 Down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
title_sort ab283. spr-10 down-regulation of ryanodine receptor gene expression in murine urinary bladder smooth muscle following partial bladder outlet obstruction
topic Abstract
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5143274/
http://dx.doi.org/10.21037/tau.2016.s283
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