TY - JOUR
T1 - Chlamydia Trachomatis in vivo to in vitro transition reveals mechanisms of phase variation and down-regulation of virulence factors
AU - Borges, Vítor
AU - Pinheiro, Miguel
AU - Antelo, Minia
AU - Sampaio, Daniel A.
AU - Vieira, Luís
AU - Ferreira, Rita
AU - Nunes, Alexandra
AU - Almeida, Filipe
AU - Mota, Luís J.
AU - Borrego, Maria J.
AU - Gomes, João Paulo
N1 - Fundacao para a Ciencia e a Tecnologia (FCT) (SFRH/BD/68527/2010);
Wellcome Trust ISSF grant (097831/Z/11/Z);
FCT (SFRH/BD/68532/2010; SFRH/BPD/75295/2010)
PY - 2015/7/24
Y1 - 2015/7/24
N2 - Research on the obligate intracellular bacterium Chlamydia trachomatis demands culture in cell-lines, but the adaptive process behind the in vivo to in vitro transition is not understood. We assessed the genomic and transcriptomic dynamics underlying C.Trachomatis in vitro adaptation of strains representing the three disease groups (ocular, epithelial-genital and lymphogranuloma venereum) propagated in epithelial cells over multiple passages.We found genetic features potentially underlying phase variation mechanisms mediating the regulation of a lipid A biosynthesis enzyme (CT533/LpxC), and the functionality of the cytotoxin (CT166) through an ON/OFF mechanism. We detected inactivating mutations in CT713/porB, a scenario suggesting metabolic adaptation to the available carbon source. CT135 was inactivated in a tropism-specific manner, with CT135-negative clones emerging for all epithelial-genital populations (but not for LGV and ocular populations) and rapidly increasing in frequency (~23%mutants per10 passages). RNA-sequencing analyses revealed that a deletion event involving CT135 impacted the expression of multiple virulence factors, namely effectors known to play a role in the C.Trachomatis host-cell invasion or subversion (e.g., CT456/Tarp, CT694, CT875/TepP and CT868/ChlaDub1). This reflects a scenario of attenuation of C.Trachomatis virulence in vitro, which may take place independently or in a cumulative fashion with the also observed down-regulation of plasmid-related virulence factors. This issue may be relevant on behalf of the recent advances in Chlamydia mutagenesis and transformation where culture propagation for selecting mutants/transformants is mandatory. Finally, there was an increase in the growth rate for all strains, reflecting gradual fitness enhancement over time. In general, these data shed light on the adaptive process underlying the C.Trachomatis in vivo to in vitro transition, and indicates that it would be prudent to restrict culture propagation to minimal passages and check the status of the CT135 genotype in order to avoid the selection of CT135-negative mutants, likely originating less virulent strains.
AB - Research on the obligate intracellular bacterium Chlamydia trachomatis demands culture in cell-lines, but the adaptive process behind the in vivo to in vitro transition is not understood. We assessed the genomic and transcriptomic dynamics underlying C.Trachomatis in vitro adaptation of strains representing the three disease groups (ocular, epithelial-genital and lymphogranuloma venereum) propagated in epithelial cells over multiple passages.We found genetic features potentially underlying phase variation mechanisms mediating the regulation of a lipid A biosynthesis enzyme (CT533/LpxC), and the functionality of the cytotoxin (CT166) through an ON/OFF mechanism. We detected inactivating mutations in CT713/porB, a scenario suggesting metabolic adaptation to the available carbon source. CT135 was inactivated in a tropism-specific manner, with CT135-negative clones emerging for all epithelial-genital populations (but not for LGV and ocular populations) and rapidly increasing in frequency (~23%mutants per10 passages). RNA-sequencing analyses revealed that a deletion event involving CT135 impacted the expression of multiple virulence factors, namely effectors known to play a role in the C.Trachomatis host-cell invasion or subversion (e.g., CT456/Tarp, CT694, CT875/TepP and CT868/ChlaDub1). This reflects a scenario of attenuation of C.Trachomatis virulence in vitro, which may take place independently or in a cumulative fashion with the also observed down-regulation of plasmid-related virulence factors. This issue may be relevant on behalf of the recent advances in Chlamydia mutagenesis and transformation where culture propagation for selecting mutants/transformants is mandatory. Finally, there was an increase in the growth rate for all strains, reflecting gradual fitness enhancement over time. In general, these data shed light on the adaptive process underlying the C.Trachomatis in vivo to in vitro transition, and indicates that it would be prudent to restrict culture propagation to minimal passages and check the status of the CT135 genotype in order to avoid the selection of CT135-negative mutants, likely originating less virulent strains.
KW - OBLIGATE INTRACELLULAR PATHOGEN
KW - GUANYLATE BINDING-PROTEINS
KW - III SECRETION MECHANISM
KW - EARLY-CYCLE DEVELOPMENT
KW - OUTER-MEMBRANE COMPLEX
KW - HISTONE-LIKE PROTEIN
KW - MESSENGER-RNA DECAY
KW - KAPPA-B PATHWAY
KW - LYMPHOGRANULOMA-VENEREUM
KW - ESCHERICHIA-COLI
UR - http://www.scopus.com/inward/record.url?scp=84941712082&partnerID=8YFLogxK
U2 - 10.1371/journal.pone.0133420
DO - 10.1371/journal.pone.0133420
M3 - Article
C2 - 26207372
AN - SCOPUS:84941712082
SN - 1932-6203
VL - 10
JO - PLoS ONE
JF - PLoS ONE
IS - 7
M1 - e0133420
ER -