Mondeja B A, Jensen J S, Rodríguez I, Morier L F, Kourí V, Rodríguez N M, Fernández C
National Reference Laboratory of Mycoplasmas Research, "Pedro Kourí" Tropical Medicine Institute (IPK) Havana, Cuba.
Mycoplasma Laboratory, Staten Serum Institut Copenhagen, Denmark.
New Microbes New Infect. 2013 Nov;1(2):22-6. doi: 10.1002/2052-2975.20. Epub 2013 Nov 28.
Isolation of Mycoplasma genitalium from clinical specimens remains difficult. We describe a modified culture system based on Vero cells grown in medium 199 with 2% foetal bovine serum (FBS). The culture system was evaluated using early passage M. genitalium strains M6271 and M6311 with growth monitoring by quantitative TaqMan PCR. Eleven endocervical swabs and one male urethral swab positive by 16S rRNA and MgPa1-3 PCRs were quantified and inoculated into Vero cell suspensions in medium 199 supplemented with 2% FBS and antibiotics. Cultures were incubated for 14 days. Cell passages and growth monitoring by TaqMan PCR were performed until the growth of M. genitalium reached ≥10(6) geq/mL. Confirmation of the new M. genitalium strains was performed by sequencing a 281 bp fragment of mgpB. The growth of Mycoplasma genitalium strains was recorded for all urogenital swab specimens in the modified cell-culture system. Growth of M. genitalium was obtained within 2 months and yielded 12 M. genitalium strains with all 11 isolates from females of an identical, but unique genotype. To our knowledge, this is the first successful isolation of M. genitalium in the Latin-American region. The use of Vero cell culture in 199 medium with 2% FBS is a method comparable to the Ultroser G culture system for isolation of M. genitalium. Genotyping of clinical samples and isolates should be performed to document the absence of cross-contamination.
从临床标本中分离生殖支原体仍然困难。我们描述了一种基于在含有2%胎牛血清(FBS)的199培养基中生长的Vero细胞的改良培养系统。使用早期传代的生殖支原体菌株M6271和M6311对该培养系统进行评估,并通过定量TaqMan PCR监测生长情况。对11份经16S rRNA和MgPa1 - 3 PCR检测呈阳性的宫颈拭子和1份男性尿道拭子进行定量,并接种到添加了2% FBS和抗生素的199培养基中的Vero细胞悬液中。培养14天。通过TaqMan PCR进行细胞传代和生长监测,直至生殖支原体的生长达到≥10(6) geq/mL。通过对mgpB的281 bp片段进行测序来确认新的生殖支原体菌株。在改良的细胞培养系统中记录了所有泌尿生殖拭子标本中生殖支原体菌株的生长情况。在2个月内获得了生殖支原体的生长,并产生了12株生殖支原体菌株,其中11株来自女性的分离株具有相同但独特的基因型。据我们所知,这是拉丁美洲地区首次成功分离出生殖支原体。在含有2% FBS的199培养基中使用Vero细胞培养是一种与用于分离生殖支原体的Ultroser G培养系统相当的方法。应对临床样本和分离株进行基因分型,以证明不存在交叉污染。
