Development of a small shuttle plasmid for use in oral Veillonella and initial appraisal of potential for fluorescence-based applications

维管菌 穿梭机载体 质粒 生物 微生物学 细菌 遗传学 重组DNA DNA 载体(分子生物学) 基因 链球菌
作者
M. Paula Goetting‐Minesky,J H Kim,Duane T White,Michael A. L. Hayashi,Alexander H. Rickard,J. Christopher Fenno
出处
期刊:Letters in Applied Microbiology [Oxford University Press]
卷期号:77 (8) 被引量:1
标识
DOI:10.1093/lambio/ovae069
摘要

Abstract Oral Veillonella species are among the early colonizers of the human oral cavity. We constructed a small, single-selectable-marker shuttle plasmid, examined its ability to be transformed into diverse oral Veillonella strains, and assessed its potential use for expressing a gene encoding an oxygen-independent fluorescent protein, thus generating a fluorescent Veillonella parvula strain. Because tetracycline resistance is common in Veillonella, we replaced genes encoding ampicillin- and tetracycline-resistance in a previously described shuttle plasmid (pBSJL2) with a chloramphenicol acetyltransferase gene. The resulting plasmid pCF1135 was successfully introduced into four strains representing V. parvula and V. atypica by either natural transformation or electroporation. We then modified this plasmid to express a gene encoding an oxygen-independent fluorescent protein in V. parvula SKV38. The resulting strain yielded a fluorescence signal intensity ∼16 times higher than the wild type in microplate-based fluorimetry experiments. While fluorescence microscopy demonstrated that planktonic cells, colonies, and biofilms of fluorescent V. parvula could also be imaged, photobleaching was a significant issue. In conclusion, we anticipate this genetic system and information provided here will facilitate expanded studies of oral Veillonella species’ properties and behavior.
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