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Strain-dependent host transcriptional responses to toxoplasma infection are largely conserved in mammalian and avian hosts
Authors
A Khaminets
A Khan
+59 more
A Khan
A Subramanian
AI Saeed
AM Pollard
B Gajria
CA Dobbin
CN Kaneto
D Ajzenberg
DS Roos
DV Pechkovsky
EE Rosowski
G Dennis Jr
GS Yap
IJ Blader
J Laliberté
JC Boothroyd
John C. Boothroyd
Jon P. Boyle
JP Boyle
JP Dubey
JP Dubey
JP Dubey
JP Dubey
JP Saeij
JPJ Saeij
JPJ Saeij
JS Stumhofer
K Friedrich
KD Jensen
KW Broman
L Peixoto
LG Rahme
M Kieslinger
M Yamamoto
M Yamamoto
MA Miller
MB Angeloni
ME Grigg
Mohamed-Ali Hakimi
P Jourdan
P Kaiser
P Kaiser
PM Robben
R Hernandez
R Irizarry
RS Lewis
RT Gazzinelli
S Hemmers
S Mitra
S Taylor
SJ Fentress
T Ikeda
T Steinfeldt
VG Tusher
VK Mootha
W Huang da
X Xie
YC Ong
Yi-Ching Ong
Publication date
1 October 2011
Publisher
'Public Library of Science (PLoS)'
Doi
View
on
PubMed
Abstract
Toxoplasma gondii has a remarkable ability to infect an enormous variety of mammalian and avian species. Given this, it is surprising that three strains (Types I/II/III) account for the majority of isolates from Europe/North America. The selective pressures that have driven the emergence of these particular strains, however, remain enigmatic. We hypothesized that strain selection might be partially driven by adaptation of strains for mammalian versus avian hosts. To test this, we examine in vitro, strain-dependent host responses in fibroblasts of a representative avian host, the chicken (Gallus gallus). Using gene expression profiling of infected chicken embryonic fibroblasts and pathway analysis to assess host response, we show here that chicken cells respond with distinct transcriptional profiles upon infection with Type II versus III strains that are reminiscent of profiles observed in mammalian cells. To identify the parasite drivers of these differences, chicken fibroblasts were infected with individual F1 progeny of a Type II x III cross and host gene expression was assessed for each by microarray. QTL mapping of transcriptional differences suggested, and deletion strains confirmed, that, as in mammalian cells, the polymorphic rhoptry kinase ROP16 is the major driver of strain-specific responses. We originally hypothesized that comparing avian versus mammalian host response might reveal an inversion in parasite strain-dependent phenotypes; specifically, for polymorphic effectors like ROP16, we hypothesized that the allele with most activity in mammalian cells might be less active in avian cells. Instead, we found that activity of ROP16 alleles appears to be conserved across host species; moreover, additional parasite loci that were previously mapped for strain-specific effects on mammalian response showed similar strain-specific effects in chicken cells. These results indicate that if different hosts select for different parasite genotypes, the selection operates downstream of the signaling occurring during the beginning of the host's immune response. © 2011 Ong et al
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