New Recombinant Mycobacterium bovis BCG Expression Vectors: Improving Genetic Control over Mycobacterial Promoters

Alex I. Kanno; Cibelly Goulart; Henrique K. Rofatto; Sérgio C. Oliveira; L. C. C. Leite; Johnjoe McFadden

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New Recombinant Mycobacterium bovis BCG Expression Vectors: Improving Genetic Control over Mycobacterial Promoters

Alex I. Kanno ^[3] ; Cibelly Goulart ^[3] ; Henrique K. Rofatto ^[3] ; Sergio C. Oliveira ^[1] ; Luciana C. C. Leite ^[4] ; Johnjoe McFadden ^[2]
1. [1] Universidade Federal de Minas Gerais
  
  Universidade Federal de Minas Gerais
  
  Brasil
2. [2] University of Surrey
  
  University of Surrey
  
  Guildford District, Reino Unido
3. [3] aCentro de Biotecnologia, Instituto Butantan, São Paulo, SP, Brazil; bPrograma de Pós Graduação Interunidades em Biotecnologia USP-IPT-IB, São Paulo, Brazil
4. [4] aCentro de Biotecnologia, Instituto Butantan, São Paulo, SP, Brazil
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Localización: Applied and Environmental Microbiology, ISSN 0099-2240, Vol. 82, Nº 8, 2016, págs. 2240-2246
Idioma: inglés
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Resumen
- The expression of many antigens, stimulatory molecules, or even metabolic pathways in mycobacteria such as Mycobacterium bovis BCG or M. smegmatis was made possible through the development of shuttle vectors, and several recombinant vaccines have been constructed. However, gene expression in any of these systems relied mostly on the selection of natural promoters expected to provide the required level of expression by trial and error. To establish a systematic selection of promoters with a range of strengths, we generated a library of mutagenized promoters through error-prone PCR of the strong PL5 promoter, originally from mycobacteriophage L5. These promoters were cloned upstream of the enhanced green fluorescent protein reporter gene, and recombinant M. smegmatis bacteria exhibiting a wide range of fluorescence levels were identified. A set of promoters was selected and identified as having high (pJK-F8), intermediate (pJK-B7, pJK-E6, pJK-D6), or low (pJK-C1) promoter strengths in both M. smegmatis and M. bovis BCG. The sequencing of the promoter region demonstrated that it was extensively modified (6 to 11%) in all of the plasmids selected. To test the functionality of the system, two different expression vectors were demonstrated to allow corresponding expression levels of the Schistosoma mansoni antigen Sm29 in BCG. The approach used here can be used to adjust expression levels for synthetic and/or systems biology studies or for vaccine development to maximize the immune response.