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The pyrE Gene as a Bidirectional Selection Marker in Bifidobacterium Longum 105-A

机译:pyrE基因作为双歧杆菌105-A中的双向选择标记

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摘要

We constructed a deletion mutant of the pyrE gene in Bifidobacterium longum 105-A. A pyrE knockout cassette was cloned into pKKT427, a Bifidobacterium-Escherichia coli shuttle vector, and then introduced into B. longum 105-A by electroporation. The transformants were propagated and spread onto MRS plates containing 5-fluoroorotic acid (5-FOA) and uracil. 5-FOA-resistant mutants were obtained at a frequency of 4.7 × 10−5 integrations per cell. To perform pyrE gene complementation, the pyrE gene was amplified by PCR and used to construct a complementation plasmid (pKKT427-pyrE+). B. longum 105-A ∆pyrE harboring this plasmid could not grow on MRS plates containing 5-FOA, uracil and spectinomycin. We also developed a chemically defined medium (bifidobacterial minimal medium; BMM) containing inorganic salts, glucose, vitamins, isoleucine and tyrosine for positive selection of pyrE transformants. B. longum 105-A ∆pyrE could not grow on BMM agar, but the same strain harboring pKKT427-pyrE+ could. Thus, pyrE can be used as a counterselection marker inB. longum 105-A and potentially other Bifidobacteriumspecies as well. We demonstrated the effectiveness of this system by constructing aknockout mutant of the xynF gene in B. longum 105-A byusing the pyrE gene as a counterselection marker. ThispyrE-based selection system will contribute to genetic studies ofbifidobacteria.
机译:我们在长双歧杆菌105-A中构建了pyrE基因的缺失突变体。将pyrE基因敲除盒克隆到双歧杆菌-大肠杆菌穿梭载体pKKT427中,然后通过电穿孔引入长双歧杆菌105-A中。使转化体繁殖并铺展到含有5-氟乳清酸(5-FOA)和尿嘧啶的MRS平板上。以每个细胞4.7×10 -5 整合的频率获得了5-FOA抗性突变体。为了进行pyrE基因的互补,通过PCR扩增了pyrE基因,并用于构建互补质粒(pKKT427-pyrE + )。带有该质粒的长双歧杆菌105-AΔpyrE不能在含有5-FOA,尿嘧啶和大观霉素的MRS平板上生长。我们还开发了化学定义的培养基(双歧杆菌基本培养基; BMM),其中含有无机盐,葡萄糖,维生素,异亮氨酸和酪氨酸,可用于积极选择pyrE转化子。 B.longum 105-AΔpyrE不能在BMM琼脂上生长,但是带有pKKT427-pyrE + 的同一菌株可以生长。因此,pyrE可以用作反选择标记 B。 longum 105-A和其他可能的双歧杆菌种类也是如此。我们通过构建一个 B中 xynF 基因的敲除突变体。 longum 105-A由使用 pyrE 基因作为反选择标记。这个基于 pyrE 的选择系统将有助于对双歧杆菌。

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