A. Library preparation strategy: poly-A(+) RNAs are captured by complementarity to reverse transcription primer, then second strand is synthesized using random hexamers and handles for sequencing are attached through two rounds of PCR. B. Mapped read distribution by species and by biotype. C and D. Principal component analysis of mouse and <i>T. gondii</i> transcriptomes, respectively. E and F. Volcano plots of Live <i>Toxoplasma</i>-infected mouse and <i>T. gondii</i> time points, respectively. To calculate Log<sub>2</sub>(Fold change), every timepoint is compared to corresponding samples (either macrophage or <i>Toxoplasma</i>) before infection (t = 0 min). Most significant and most upregulated transcripts are labelled. Number of significantly (p ≤ 0.05) downregulated and upregulated genes for each time point is given in blue and red, respectively. In F, 24-hour time point, red dots mark ROP

A. Library preparation strategy: poly-A(+) RNAs are captured by complementarity to reverse transcription primer, then second strand is synthesized using random hexamers and handles for sequencing are attached through two rounds of PCR. B. Mapped read distribution by species and by biotype. C and D. Principal component analysis of mouse and <i>T. gondii</i> transcriptomes, respectively. E and F. Volcano plots of Live <i>Toxoplasma</i>-infected mouse and <i>T. gondii</i> time points, respectively. To calculate Log<sub>2</sub>(Fold change), every timepoint is compared to corresponding samples (either macrophage or <i>Toxoplasma</i>) before infection (t = 0 min). Most significant and most upregulated transcripts are labelled. Number of significantly (p ≤ 0.05) downregulated and upregulated genes for each time point is given in blue and red, respectively. In F, 24-hour time point, red dots mark ROP

<p>A. Library preparation strategy: poly-A(+) RNAs are captured by complementarity to reverse transcription primer, then second strand is synthesized using random hexamers and handles for sequencing are attached through two rounds of PCR. B. Mapped read distribution by species and by biotype....

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Dades bibliogràfiques
Autor principal: Dominykas Murza (22676289) (author)
Altres autors: Filip Lastovka (22676292) (author), George Wood (7488866) (author), Matthew P. Brember (12780473) (author), Oliver Chan (22676295) (author), James W. Ajioka (9255) (author), Betty Y. W. Chung (22676298) (author)
Publicat: 2025
Matèries:
Microbiology
Cell Biology
Immunology
Developmental Biology
Science Policy
Infectious Diseases
Environmental Sciences not elsewhere classified
Biological Sciences not elsewhere classified
Physical Sciences not elsewhere classified
resolved transcriptomic profiling
leveraging inactivated parasites
initial triggers shaping
immune system ’
immune suppressors dominates
even behavioural changes
div >< p
strategic transcriptional shift
live infection —
earliest transcriptional shifts
determining infection outcomes
general immune activation
toxoplasma gondii </
gondii </
transcriptional level
infection model
delayed activation
using time
study unveils
secreted proteins
pivotal role
parasite secures
mouse macrophage
master manipulator
macrophage response
increased suppressor
hormone disruption
growth capacity
first responders
first line
findings reveal
early upregulation
early increase
disentangled responses
delayed strategy
apicomplexan parasite
active invasion
7 -<
60 minutes
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