Estrogen modulates the expression of myosin heavy chain in detrusor smooth muscle

Ricardo F. Sánchez-Ortiz; Ze Wang; Chandrakala Menon; Michael E. DiSanto; Alan J. Wein; Samuel Chacko

doi:10.1152/ajpcell.2001.280.3.c433

Estrogen modulates the expression of myosin heavy chain in detrusor smooth muscle

Ricardo F. Sánchez-Ortiz
, Ze Wang
, Chandrakala Menon
, Michael E. DiSanto
, Alan J. Wein
, Samuel Chacko

Research output: Contribution to journal › Article › peer-review

29 Scopus citations

Abstract

The effect of low serum estrogen levels on urinary bladder function remains poorly understood. Using a rabbit model, we analyzed the effects of estrogen on the expression of the isoforms of myosin, the molecular motor for muscle contraction, in detrusor smooth muscle. Expression of myosin heavy chain (MHC) isoforms, which differ in the COOH-terminal (SM1 and SM2) and the NH₂terminal (SM-A and SM-B) regions as a result of alternative splicing of the mRNA at either the 3′- or 5′-ends, was analyzed in age-matched female rabbits that were sham operated, ovariectomized (Ovx), and given estrogen after ovariectomy (4 rabbits/group). Ovx rabbits showed a significant decrease in the overall MHC content per gram of wet detrusor smooth muscle compared with controls (P < 0.04), which was reversed by estrogen replacement (P < 0.02). MHC content, as a proportion of total milligram of protein in the bladder tissue extracted, was also increased in estrogentreated Ovx rabbits. Quantitative competitive RT-PCR revealed 1.72-, 2.63-, and 5.82 × 10⁶ copies of MHC mRNA/100 ng total mRNA in Ovx, control, and estrogen-treated rabbits, respectively (P < 0.01). RT-PCR analysis using oligonucleotides specific for the region containing the SM1/SM2 MHC alternative splice sites indicated a lower SM2-to-SM1 ratio in estrogen-treated compared with control and Ovx rabbits (P < 0.05). Similarly, SDS-PAGE analysis of extracted myosin from estrogen-treated rabbits revealed a significantly lower SM2-to-SM1 isoform ratio compared with control and Ovx rabbits (P < 0.05). Expression of the SM-A and SM-B isoforms was not affected. These results indicate that myosin content is increased upon estrogen replacement in Ovx rabbits and that the abundance of SM1 relative to SM2 is greater in estrogen-treated rabbits compared with normal and Ovx rabbits. These data suggest that estrogen affects alternative splicing at the 3′-end of the MHC pre-mRNA to increase the proportion of SM1 vs. SM2.

Original language	English (US)
Pages (from-to)	C433-C440
Journal	American Journal of Physiology - Cell Physiology
Volume	280
Issue number	3 49-3
DOIs	https://doi.org/10.1152/ajpcell.2001.280.3.c433
State	Published - 2001
Externally published	Yes

All Science Journal Classification (ASJC) codes

Physiology
Cell Biology

Access to Document

10.1152/ajpcell.2001.280.3.c433

Cite this

@article{62a0ffb1df02473d943789428b99eba0,

title = "Estrogen modulates the expression of myosin heavy chain in detrusor smooth muscle",

abstract = "The effect of low serum estrogen levels on urinary bladder function remains poorly understood. Using a rabbit model, we analyzed the effects of estrogen on the expression of the isoforms of myosin, the molecular motor for muscle contraction, in detrusor smooth muscle. Expression of myosin heavy chain (MHC) isoforms, which differ in the COOH-terminal (SM1 and SM2) and the NH2terminal (SM-A and SM-B) regions as a result of alternative splicing of the mRNA at either the 3′- or 5′-ends, was analyzed in age-matched female rabbits that were sham operated, ovariectomized (Ovx), and given estrogen after ovariectomy (4 rabbits/group). Ovx rabbits showed a significant decrease in the overall MHC content per gram of wet detrusor smooth muscle compared with controls (P < 0.04), which was reversed by estrogen replacement (P < 0.02). MHC content, as a proportion of total milligram of protein in the bladder tissue extracted, was also increased in estrogentreated Ovx rabbits. Quantitative competitive RT-PCR revealed 1.72-, 2.63-, and 5.82 × 106 copies of MHC mRNA/100 ng total mRNA in Ovx, control, and estrogen-treated rabbits, respectively (P < 0.01). RT-PCR analysis using oligonucleotides specific for the region containing the SM1/SM2 MHC alternative splice sites indicated a lower SM2-to-SM1 ratio in estrogen-treated compared with control and Ovx rabbits (P < 0.05). Similarly, SDS-PAGE analysis of extracted myosin from estrogen-treated rabbits revealed a significantly lower SM2-to-SM1 isoform ratio compared with control and Ovx rabbits (P < 0.05). Expression of the SM-A and SM-B isoforms was not affected. These results indicate that myosin content is increased upon estrogen replacement in Ovx rabbits and that the abundance of SM1 relative to SM2 is greater in estrogen-treated rabbits compared with normal and Ovx rabbits. These data suggest that estrogen affects alternative splicing at the 3′-end of the MHC pre-mRNA to increase the proportion of SM1 vs. SM2.",

author = "S{\'a}nchez-Ortiz, \{Ricardo F.\} and Ze Wang and Chandrakala Menon and DiSanto, \{Michael E.\} and Wein, \{Alan J.\} and Samuel Chacko",

year = "2001",

doi = "10.1152/ajpcell.2001.280.3.c433",

language = "English (US)",

volume = "280",

pages = "C433--C440",

journal = "American Journal of Physiology - Cell Physiology",

issn = "0363-6143",

publisher = "American Physiological Society",

number = "3 49-3",

}

TY - JOUR

T1 - Estrogen modulates the expression of myosin heavy chain in detrusor smooth muscle

AU - Sánchez-Ortiz, Ricardo F.

AU - Wang, Ze

AU - Menon, Chandrakala

AU - DiSanto, Michael E.

AU - Wein, Alan J.

AU - Chacko, Samuel

PY - 2001

Y1 - 2001

N2 - The effect of low serum estrogen levels on urinary bladder function remains poorly understood. Using a rabbit model, we analyzed the effects of estrogen on the expression of the isoforms of myosin, the molecular motor for muscle contraction, in detrusor smooth muscle. Expression of myosin heavy chain (MHC) isoforms, which differ in the COOH-terminal (SM1 and SM2) and the NH2terminal (SM-A and SM-B) regions as a result of alternative splicing of the mRNA at either the 3′- or 5′-ends, was analyzed in age-matched female rabbits that were sham operated, ovariectomized (Ovx), and given estrogen after ovariectomy (4 rabbits/group). Ovx rabbits showed a significant decrease in the overall MHC content per gram of wet detrusor smooth muscle compared with controls (P < 0.04), which was reversed by estrogen replacement (P < 0.02). MHC content, as a proportion of total milligram of protein in the bladder tissue extracted, was also increased in estrogentreated Ovx rabbits. Quantitative competitive RT-PCR revealed 1.72-, 2.63-, and 5.82 × 106 copies of MHC mRNA/100 ng total mRNA in Ovx, control, and estrogen-treated rabbits, respectively (P < 0.01). RT-PCR analysis using oligonucleotides specific for the region containing the SM1/SM2 MHC alternative splice sites indicated a lower SM2-to-SM1 ratio in estrogen-treated compared with control and Ovx rabbits (P < 0.05). Similarly, SDS-PAGE analysis of extracted myosin from estrogen-treated rabbits revealed a significantly lower SM2-to-SM1 isoform ratio compared with control and Ovx rabbits (P < 0.05). Expression of the SM-A and SM-B isoforms was not affected. These results indicate that myosin content is increased upon estrogen replacement in Ovx rabbits and that the abundance of SM1 relative to SM2 is greater in estrogen-treated rabbits compared with normal and Ovx rabbits. These data suggest that estrogen affects alternative splicing at the 3′-end of the MHC pre-mRNA to increase the proportion of SM1 vs. SM2.

AB - The effect of low serum estrogen levels on urinary bladder function remains poorly understood. Using a rabbit model, we analyzed the effects of estrogen on the expression of the isoforms of myosin, the molecular motor for muscle contraction, in detrusor smooth muscle. Expression of myosin heavy chain (MHC) isoforms, which differ in the COOH-terminal (SM1 and SM2) and the NH2terminal (SM-A and SM-B) regions as a result of alternative splicing of the mRNA at either the 3′- or 5′-ends, was analyzed in age-matched female rabbits that were sham operated, ovariectomized (Ovx), and given estrogen after ovariectomy (4 rabbits/group). Ovx rabbits showed a significant decrease in the overall MHC content per gram of wet detrusor smooth muscle compared with controls (P < 0.04), which was reversed by estrogen replacement (P < 0.02). MHC content, as a proportion of total milligram of protein in the bladder tissue extracted, was also increased in estrogentreated Ovx rabbits. Quantitative competitive RT-PCR revealed 1.72-, 2.63-, and 5.82 × 106 copies of MHC mRNA/100 ng total mRNA in Ovx, control, and estrogen-treated rabbits, respectively (P < 0.01). RT-PCR analysis using oligonucleotides specific for the region containing the SM1/SM2 MHC alternative splice sites indicated a lower SM2-to-SM1 ratio in estrogen-treated compared with control and Ovx rabbits (P < 0.05). Similarly, SDS-PAGE analysis of extracted myosin from estrogen-treated rabbits revealed a significantly lower SM2-to-SM1 isoform ratio compared with control and Ovx rabbits (P < 0.05). Expression of the SM-A and SM-B isoforms was not affected. These results indicate that myosin content is increased upon estrogen replacement in Ovx rabbits and that the abundance of SM1 relative to SM2 is greater in estrogen-treated rabbits compared with normal and Ovx rabbits. These data suggest that estrogen affects alternative splicing at the 3′-end of the MHC pre-mRNA to increase the proportion of SM1 vs. SM2.

UR - https://www.scopus.com/pages/publications/0034996368

UR - https://www.scopus.com/pages/publications/0034996368#tab=citedBy

U2 - 10.1152/ajpcell.2001.280.3.c433

DO - 10.1152/ajpcell.2001.280.3.c433

M3 - Article

C2 - 11171561

AN - SCOPUS:0034996368

SN - 0363-6143

VL - 280

SP - C433-C440

JO - American Journal of Physiology - Cell Physiology

JF - American Journal of Physiology - Cell Physiology

IS - 3 49-3

ER -

Estrogen modulates the expression of myosin heavy chain in detrusor smooth muscle

Abstract

All Science Journal Classification (ASJC) codes

Access to Document

Other files and links

Fingerprint

Cite this