Establishment of a transgenic sickle-cell mouse model to study the pathophysiology of priapism

Trinity J. Bivalacqua; Biljana Musicki; Lewis L. Hsu; Mark T. Gladwin; Arthur L. Burnett; Hunter C. Champion

doi:10.1111/j.1743-6109.2009.01359.x

Establishment of a transgenic sickle-cell mouse model to study the pathophysiology of priapism

Trinity J. Bivalacqua, Biljana Musicki, Lewis L. Hsu, Mark T. Gladwin, Arthur L. Burnett, Hunter C. Champion

School of Medicine

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

48 Scopus citations

Abstract

Introduction. Priapism is a poorly understood disease process with little information on the etiology and pathophysiology of this erectile disorder. One group of patients with a high prevalence of priapism is men with sickle-cell disease. Aim. Establish an in vivo transgenic sickle-cell mouse model to study the pathophysiology of sickle-cell disease-associated priapism. Methods. Transgenic sickle-cell disease mice, expressing human sickle hemoglobin, were utilized. Three groups of mice were used: (i) wild type (WT), (ii) sickle-cell heterozygotes (Hemi), and (ii) sickle-cell homozygotes (Sickle). Two age groups of each cohort of mice were utilized: young adult (4-6 months) and aged (18-22 months). Main Outcome Measures. Histological (trichrome stain to measure ratio of collagen to smooth muscle), penile hydroxyproline content (collagen content), and transmission electron microscopic analysis of WT, Hemi, and Sickle mice penes, as well as in vivo erectile responses [change in intracavernous pressure (ICP)]to cavernous nerve stimulation (CNS), were determined. The frequency of erectile responses (erections/hour) pre- and poststimulation was also measured in each of the experimental groups. Results. Sickle mice had increased (P < 0.05) collagen to smooth muscle ratio and hydroxyproline content in the penis when compared with WT and Hemi mice penes. Transmission electron microscopy demonstrated thickened smooth muscle cell bundles, disruption of the endothelial lining of the corporal sinusoids, and increased (P < 0.05) caveolae number. Sickle mice had significantly (P < 0.05) higher ICP to CNS and increased (P < 0.05) frequency of erections pre- and post-CNS when compared with WT and Hemi mice erectile responses. Sickle mice did develop ED (change in ICP in response to CNS) with increasing age. Conclusion. The morphometric changes of the penis and exaggerated in vivo erectile responses support the use of this transgenic sickle-cell disease animal model to study the pathophysiological mechanisms involved in sickle-cell disease-associated priapism.

Original language	English (US)
Pages (from-to)	2494-2504
Number of pages	11
Journal	Journal of Sexual Medicine
Volume	6
Issue number	9
DOIs	https://doi.org/10.1111/j.1743-6109.2009.01359.x
State	Published - 2009

Keywords

Cavolae
Endothelium
Erectile Dysfunction
Fibrosis
Ischemic Priapism
Nitric Oxide

ASJC Scopus subject areas

General Medicine

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10.1111/j.1743-6109.2009.01359.x

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@article{f7700c5c05dc4721967cbe361109a582,

title = "Establishment of a transgenic sickle-cell mouse model to study the pathophysiology of priapism",

abstract = "Introduction. Priapism is a poorly understood disease process with little information on the etiology and pathophysiology of this erectile disorder. One group of patients with a high prevalence of priapism is men with sickle-cell disease. Aim. Establish an in vivo transgenic sickle-cell mouse model to study the pathophysiology of sickle-cell disease-associated priapism. Methods. Transgenic sickle-cell disease mice, expressing human sickle hemoglobin, were utilized. Three groups of mice were used: (i) wild type (WT), (ii) sickle-cell heterozygotes (Hemi), and (ii) sickle-cell homozygotes (Sickle). Two age groups of each cohort of mice were utilized: young adult (4-6 months) and aged (18-22 months). Main Outcome Measures. Histological (trichrome stain to measure ratio of collagen to smooth muscle), penile hydroxyproline content (collagen content), and transmission electron microscopic analysis of WT, Hemi, and Sickle mice penes, as well as in vivo erectile responses [change in intracavernous pressure (ICP)]to cavernous nerve stimulation (CNS), were determined. The frequency of erectile responses (erections/hour) pre- and poststimulation was also measured in each of the experimental groups. Results. Sickle mice had increased (P < 0.05) collagen to smooth muscle ratio and hydroxyproline content in the penis when compared with WT and Hemi mice penes. Transmission electron microscopy demonstrated thickened smooth muscle cell bundles, disruption of the endothelial lining of the corporal sinusoids, and increased (P < 0.05) caveolae number. Sickle mice had significantly (P < 0.05) higher ICP to CNS and increased (P < 0.05) frequency of erections pre- and post-CNS when compared with WT and Hemi mice erectile responses. Sickle mice did develop ED (change in ICP in response to CNS) with increasing age. Conclusion. The morphometric changes of the penis and exaggerated in vivo erectile responses support the use of this transgenic sickle-cell disease animal model to study the pathophysiological mechanisms involved in sickle-cell disease-associated priapism.",

keywords = "Cavolae, Endothelium, Erectile Dysfunction, Fibrosis, Ischemic Priapism, Nitric Oxide",

author = "Bivalacqua, {Trinity J.} and Biljana Musicki and Hsu, {Lewis L.} and Gladwin, {Mark T.} and Burnett, {Arthur L.} and Champion, {Hunter C.}",

note = "Funding Information: The authors would like to thank Dr. Janice Taube, Warren Mason, and Carol Cooke for their help with analysis of trichrome stain and electron microscopy of the mice penes. Dr. Bivalacqua is supported by an American Urological Association (AUA) Foundation Astellas USA Foundation MD/PhD Fellowship and recipient of a National Kidney Foundation of Maryland Research Grant. Dr. Champion is supported in part by the Bernard A. and Rebecca S. Bernard Foundation, a Scientist Development Grant from the American Heart Association, the WW Smith Foundation, and NIH P50 Hl084946. He is a Recipient of the Zipes Distinguished Young Investigator Award of the American College of Cardiology, the Shin Chun-Wang Young Investigator Award and the Giles F. Filley Memorial Award from the American Physiological Society. Dr. Burnett is supported in part from NIH RO1 DK067223 and U54HL090515. Dr. Hsu and Gladwin are supported in part by federal funds from National Cancer Institute, NIH, under contract NO1-CO-12400 and the Intramural Program of the Vascular Medicine Branch of the National Heart, Lung, and Blood Institute of the NIH. The content of the article does not necessarily reflect the views or policies of the Department of Health and Human Services, nor does mention of trade names, commercial products, or organizations imply endorsement by the U.S. government. ",

year = "2009",

doi = "10.1111/j.1743-6109.2009.01359.x",

language = "English (US)",

volume = "6",

pages = "2494--2504",

journal = "Journal of Sexual Medicine",

issn = "1743-6095",

publisher = "Wiley-Blackwell",

number = "9",

}

TY - JOUR

T1 - Establishment of a transgenic sickle-cell mouse model to study the pathophysiology of priapism

AU - Bivalacqua, Trinity J.

AU - Musicki, Biljana

AU - Hsu, Lewis L.

AU - Gladwin, Mark T.

AU - Burnett, Arthur L.

AU - Champion, Hunter C.

N1 - Funding Information: The authors would like to thank Dr. Janice Taube, Warren Mason, and Carol Cooke for their help with analysis of trichrome stain and electron microscopy of the mice penes. Dr. Bivalacqua is supported by an American Urological Association (AUA) Foundation Astellas USA Foundation MD/PhD Fellowship and recipient of a National Kidney Foundation of Maryland Research Grant. Dr. Champion is supported in part by the Bernard A. and Rebecca S. Bernard Foundation, a Scientist Development Grant from the American Heart Association, the WW Smith Foundation, and NIH P50 Hl084946. He is a Recipient of the Zipes Distinguished Young Investigator Award of the American College of Cardiology, the Shin Chun-Wang Young Investigator Award and the Giles F. Filley Memorial Award from the American Physiological Society. Dr. Burnett is supported in part from NIH RO1 DK067223 and U54HL090515. Dr. Hsu and Gladwin are supported in part by federal funds from National Cancer Institute, NIH, under contract NO1-CO-12400 and the Intramural Program of the Vascular Medicine Branch of the National Heart, Lung, and Blood Institute of the NIH. The content of the article does not necessarily reflect the views or policies of the Department of Health and Human Services, nor does mention of trade names, commercial products, or organizations imply endorsement by the U.S. government.

PY - 2009

Y1 - 2009

N2 - Introduction. Priapism is a poorly understood disease process with little information on the etiology and pathophysiology of this erectile disorder. One group of patients with a high prevalence of priapism is men with sickle-cell disease. Aim. Establish an in vivo transgenic sickle-cell mouse model to study the pathophysiology of sickle-cell disease-associated priapism. Methods. Transgenic sickle-cell disease mice, expressing human sickle hemoglobin, were utilized. Three groups of mice were used: (i) wild type (WT), (ii) sickle-cell heterozygotes (Hemi), and (ii) sickle-cell homozygotes (Sickle). Two age groups of each cohort of mice were utilized: young adult (4-6 months) and aged (18-22 months). Main Outcome Measures. Histological (trichrome stain to measure ratio of collagen to smooth muscle), penile hydroxyproline content (collagen content), and transmission electron microscopic analysis of WT, Hemi, and Sickle mice penes, as well as in vivo erectile responses [change in intracavernous pressure (ICP)]to cavernous nerve stimulation (CNS), were determined. The frequency of erectile responses (erections/hour) pre- and poststimulation was also measured in each of the experimental groups. Results. Sickle mice had increased (P < 0.05) collagen to smooth muscle ratio and hydroxyproline content in the penis when compared with WT and Hemi mice penes. Transmission electron microscopy demonstrated thickened smooth muscle cell bundles, disruption of the endothelial lining of the corporal sinusoids, and increased (P < 0.05) caveolae number. Sickle mice had significantly (P < 0.05) higher ICP to CNS and increased (P < 0.05) frequency of erections pre- and post-CNS when compared with WT and Hemi mice erectile responses. Sickle mice did develop ED (change in ICP in response to CNS) with increasing age. Conclusion. The morphometric changes of the penis and exaggerated in vivo erectile responses support the use of this transgenic sickle-cell disease animal model to study the pathophysiological mechanisms involved in sickle-cell disease-associated priapism.

AB - Introduction. Priapism is a poorly understood disease process with little information on the etiology and pathophysiology of this erectile disorder. One group of patients with a high prevalence of priapism is men with sickle-cell disease. Aim. Establish an in vivo transgenic sickle-cell mouse model to study the pathophysiology of sickle-cell disease-associated priapism. Methods. Transgenic sickle-cell disease mice, expressing human sickle hemoglobin, were utilized. Three groups of mice were used: (i) wild type (WT), (ii) sickle-cell heterozygotes (Hemi), and (ii) sickle-cell homozygotes (Sickle). Two age groups of each cohort of mice were utilized: young adult (4-6 months) and aged (18-22 months). Main Outcome Measures. Histological (trichrome stain to measure ratio of collagen to smooth muscle), penile hydroxyproline content (collagen content), and transmission electron microscopic analysis of WT, Hemi, and Sickle mice penes, as well as in vivo erectile responses [change in intracavernous pressure (ICP)]to cavernous nerve stimulation (CNS), were determined. The frequency of erectile responses (erections/hour) pre- and poststimulation was also measured in each of the experimental groups. Results. Sickle mice had increased (P < 0.05) collagen to smooth muscle ratio and hydroxyproline content in the penis when compared with WT and Hemi mice penes. Transmission electron microscopy demonstrated thickened smooth muscle cell bundles, disruption of the endothelial lining of the corporal sinusoids, and increased (P < 0.05) caveolae number. Sickle mice had significantly (P < 0.05) higher ICP to CNS and increased (P < 0.05) frequency of erections pre- and post-CNS when compared with WT and Hemi mice erectile responses. Sickle mice did develop ED (change in ICP in response to CNS) with increasing age. Conclusion. The morphometric changes of the penis and exaggerated in vivo erectile responses support the use of this transgenic sickle-cell disease animal model to study the pathophysiological mechanisms involved in sickle-cell disease-associated priapism.

KW - Cavolae

KW - Endothelium

KW - Erectile Dysfunction

KW - Fibrosis

KW - Ischemic Priapism

KW - Nitric Oxide

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Establishment of a transgenic sickle-cell mouse model to study the pathophysiology of priapism

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