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精液中细菌DNA的检测与鉴定。

Detection and identification of bacterial DNA in semen.

作者信息

Kiessling Ann A, Desmarais Bryan M, Yin Hui-Zhong, Loverde Joseph, Eyre Robert C

机构信息

Bedford Research Foundation Laboratories, Somerville, Massachusetts, USA.

出版信息

Fertil Steril. 2008 Nov;90(5):1744-56. doi: 10.1016/j.fertnstert.2007.08.083. Epub 2008 Jan 14.

Abstract

OBJECTIVE

To detect and identify bacteria in semen by sequencing polymerase chain reaction (PCR)-amplified ribosomal RNA gene regions (rDNAs).

DESIGN

Bacterial rDNAs were detected by PCR amplification of semen DNA. Conditions were adjusted to detect only abundant organisms, no fewer than 20,000 bacteria/mL of semen.

SETTING

Clinical andrology laboratory and academic research laboratories.

PATIENT(S): Men undergoing fertility evaluation (n = 29) or vasectomy (n = 5).

INTERVENTION(S): None. MAIN OUTCOME MEAURE(S): Frequency of bacterial rDNA-positive specimens, relationship of rDNAs to bacteria in GenBank, and correlation with semen cells.

RESULT(S): Twenty-five (56%) of the specimens from 22 (65%) of the men were positive. A total of 141 bacterial rDNA sequences were compared with GenBank data for identification. The largest group matched gram-positive anaerobic cocci (Peptoniphilis, Anaerococcus, Finegoldia, Peptostreptococcus spp.) in 13 specimens, followed by Corynebacterium spp. in 10 specimens, Staphylococcus, Lactobacillus, and Streptococcus spp. in 7 specimens each, Pseudomonas spp. in 4 specimens, and Haemophilus and Acinetobacter spp. in 2 specimens each. The rDNA-positive specimens averaged 59 +/- 13 million sperm/mL, 46 +/- 5% of which were motile, not statistically different from the rDNA-negative specimens (77 +/- 16 million/mL, 47 +/- 5% motile). Normal sperm forms were lower in the rDNA-positive (10 +/- 1.1%) than in the rDNA-negative specimens (22 +/- 2%), and lymphocytes/monocytes were fivefold lower in the rDNA-positive specimens (0.4 +/- 0.2 million/mL) than in the negative specimens (1.9 +/- 0.7 million/mL).

CONCLUSION(S): Abundant bacteria in semen are not commensal, arise from infection in the male genitourinary tract, may influence fertility, and may reflect an inadequate cellular immune response.

摘要

目的

通过对聚合酶链反应(PCR)扩增的核糖体RNA基因区域(rDNA)进行测序,检测和鉴定精液中的细菌。

设计

通过对精液DNA进行PCR扩增来检测细菌rDNA。调整条件以仅检测数量丰富的微生物,即每毫升精液中不少于20,000个细菌。

地点

临床男科学实验室和学术研究实验室。

患者

接受生育评估的男性(n = 29)或接受输精管切除术的男性(n = 5)。

干预措施

无。主要观察指标:细菌rDNA阳性标本的频率、rDNA与GenBank中细菌的关系以及与精液细胞的相关性。

结果

来自22名(65%)男性的25份(56%)标本呈阳性。共将141条细菌rDNA序列与GenBank数据进行比较以进行鉴定。最大的一组在13份标本中与革兰氏阳性厌氧球菌(嗜胨菌属、厌氧球菌属、费氏菌属、消化链球菌属)匹配,其次是10份标本中的棒状杆菌属,7份标本中的葡萄球菌属、乳酸杆菌属和链球菌属,4份标本中的假单胞菌属,以及每份2份标本中的嗜血杆菌属和不动杆菌属。rDNA阳性标本的平均精子浓度为59±1300万/mL,其中46±5%具有活力,与rDNA阴性标本(77±1600万/mL,47±5%具有活力)无统计学差异。rDNA阳性标本中正常精子形态(10±1.1%)低于rDNA阴性标本(22±2%),rDNA阳性标本中的淋巴细胞/单核细胞(0.4±0.2万/mL)比阴性标本(1.9±0.7万/mL)低五倍。

结论

精液中数量丰富的细菌并非共生菌,源于男性泌尿生殖道感染,可能影响生育能力,且可能反映细胞免疫反应不足。

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