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去势及睾酮替代对大鼠阴茎勃起时静脉闭塞的影响。

Effects of castration and testosterone replacement on veno-occlusion during penile erection in the rat.

作者信息

Dai Y T, Stopper V, Lewis R, Mills T

机构信息

Department of Surgery, Medical College of Georgia, Augusta 30912-3000, USA.

出版信息

Asian J Androl. 1999 Jun;1(1-2):53-9.

Abstract

AIM

To determine if androgens directly regulate veno-occlusion or if androgens act indirectly to maintain the penile structures which control outflow.

METHODS

Using CASTRATE and TESTO rats, measurement was made of mean arterial pressure (MAP), intracavernosal pressure (CCP), and intracavernosal flow (CCF) during erection resulting from stimulation of the autonomic innervation of the penis. CCP and CCF were also measured during saline infusion into the cavernosal sinuses before and after treatment with sodium nitroprusside (SNP, a nitric oxide donor drug) to fully relax cavernosal smooth muscle. Penile tissue was also collected to measure the content of alpha actin and proline and hydroxyproline to determine if brief withdrawal of androgenic support led to changes in the number of smooth muscle cells or the collagen content of the tissue.

RESULTS

Infusion of saline into the cavernosal sinuses demonstrated that veno-occlusion was defective in CASTRATE rats while veno-occlusion was fully functional in TESTO animals. Furthermore, veno-occlusion could be induced in CASTRATE rats if they were first treated with SNP. This observation suggests that failure of veno-occlusion in the CASTRATE rats is due to a deficiency in the production of NO resulting in a reduction in the degree of relaxation of the penile smooth muscle. The measurements of smooth muscle a actin and proline and hydroxyproline content of collagen showed that both were unaffected by castration and that the basic structure of the penis did not degenerate after one week without androgenic support.

CONCLUSION

These results can be interpreted to mean that androgens control the veno-occlusive mechanism indirectly via a NO dependent mechanism and not by maintaining the structures of the penis which are essential to veno-occlusion.

摘要

目的

确定雄激素是否直接调节静脉闭塞,或者雄激素是否通过间接作用来维持控制血液流出的阴茎结构。

方法

使用去势大鼠和睾酮处理大鼠,测量阴茎自主神经支配刺激引起勃起时的平均动脉压(MAP)、海绵体内压(CCP)和海绵体内血流(CCF)。在用硝普钠(SNP,一种一氧化氮供体药物)处理以完全松弛海绵体平滑肌之前和之后,在向海绵窦内注入生理盐水期间也测量CCP和CCF。还收集阴茎组织以测量α肌动蛋白以及脯氨酸和羟脯氨酸的含量,以确定短期撤除雄激素支持是否会导致平滑肌细胞数量或组织胶原蛋白含量发生变化。

结果

向海绵窦内注入生理盐水表明,去势大鼠的静脉闭塞功能存在缺陷,而睾酮处理动物的静脉闭塞功能正常。此外,如果先用SNP处理,去势大鼠可诱导出静脉闭塞。这一观察结果表明,去势大鼠静脉闭塞功能失败是由于一氧化氮产生不足,导致阴茎平滑肌松弛程度降低。平滑肌α肌动蛋白以及胶原蛋白的脯氨酸和羟脯氨酸含量的测量结果表明,两者均不受去势影响,并且在没有雄激素支持的一周后阴茎的基本结构并未退化。

结论

这些结果可以解释为,雄激素通过一氧化氮依赖性机制间接控制静脉闭塞机制,而不是通过维持对静脉闭塞至关重要的阴茎结构来实现。

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