Successful in vitro cultivation of Borrelia duttonii and its comparison with Borrelia recurrentis.

S J Cutler, C O Akintunde, J Moss, M Fukunaga, K Kurtenbach, A Talbert, H Zhang, D J Wright, D A Warrell
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引用次数: 45

Abstract

Borrelia duttonii, the cause of East African tick-borne relapsing fever, has until now been refractory to growth in laboratory media. This spirochaete has only be propagated in mice or by tissue culture, restricting both yield and purity of cells available for research. The successful isolation of five clinical isolates of B. duttonii from patients in Central Tanzania and their comparison with Borrelia recurrentis is reported. Electron microscopy revealed spirochaetal cells with pointed ends, a mean wavelength of 1.8 microns with an amplitude of 0.8 micron, similar to the findings for B. recurrentis. Cells contained 10 periplasmic flagella inserted at each end of the spirochaete, again comparable with the counts of 8-10 flagella found in B. recurrentis. PFGE revealed a chromosome of approximately 1 Mb, a large plasmid of approximately 200 kb, and a small plasmid of 11 kb in all strains of B. duttonii and in B. recurrentis. B. duttonii possessed a further 7-9 plasmids with sizes ranging from 20 to 90 kb. In two isolates of B. duttonii, the profiles were identical. In contrast, all 18 isolates of B. recurrentis fell into one of five plasmid patterns with 3-4 plasmids ranging from 25 to 61.5 kb in addition to those of 11 and 200 kb described above. Analysis of the SDS-PAGE profiles of B. duttonii strains revealed a high-molecular-mass band of 33.4-34.2 kDa in four strains (variable large protein, VLP) and a low-molecular-mass band of 22.3 kDa in the remaining strain (variable small protein, VSP). This resembles the protein profiles found in B. recurrentis. The G + C ratio of B. duttonii was 27.6 mol%. Nucleotide sequence of the rrs gene (16S rRNA) from four B. duttonii isolates revealed 100% identity among these strains and 99.7% homology with three strains deposited by others in GenBank. The rrs gene of eight representative clinical isolates of B. recurrentis confirmed their close similarity with B. duttonii.

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杜顿疏螺旋体体外培养的成功及其与复发疏螺旋体的比较。
杜氏疏螺旋体是东非蜱传回归热的病因,迄今为止在实验室培养基中难以生长。这种螺旋体只能在小鼠体内繁殖或通过组织培养,限制了可用于研究的细胞的产量和纯度。报道了从坦桑尼亚中部患者身上成功分离出的5株杜顿氏疏螺旋体临床分离株及其与复发伯氏疏螺旋体的比较。电镜显示螺旋体细胞末端呈尖状,平均波长为1.8微米,振幅为0.8微米,与B. recurtis的结果相似。在螺旋体的每一端,细胞中含有10根质周鞭毛,再次与B. recurtis中发现的8-10根鞭毛数量相当。PFGE显示,在所有duttonii菌株和复发b菌株中,都有一条约1 Mb的染色体,一个约200 kb的大质粒和一个约11 kb的小质粒。duttonii还拥有7-9个大小在20 - 90kb之间的质粒。在两个分离株中,杜氏双歧杆菌的谱图是相同的。相比之下,所有18株复发b型分离株均属于5种质粒模式之一,除了上述11和200 kb的质粒外,还有3-4个质粒在25 - 61.5 kb之间。duttonii菌株的SDS-PAGE图谱分析显示,4株菌株(可变大蛋白,VLP)具有33.4-34.2 kDa的高分子质量带,其余菌株(可变小蛋白,VSP)具有22.3 kDa的低分子质量带。这类似于在B. recurrentis中发现的蛋白谱。duttonii的G + C比为27.6 mol%。4株duttonii分离株的rrs基因(16S rRNA)核苷酸序列与其他菌株的同源性为100%,与GenBank中其他菌株的同源性为99.7%。8株具有代表性的临床分离株的rrs基因证实了它们与杜托尼布氏杆菌的密切相似性。
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