2013
DOI: 10.1242/jcs.126011
|View full text |Cite
|
Sign up to set email alerts
|

A short bifunctional element operates to positively or negatively regulateESAG9expression in different developmental forms ofTrypanosoma brucei

Abstract: SummaryIn their mammalian host trypanosomes generate 'stumpy' forms from proliferative 'slender' forms as an adaptation for transmission to their tsetse fly vector. This transition is characterised by the repression of many genes while quiescent stumpy forms accumulate during each wave of parasitaemia. However, a subset of genes are upregulated either as an adaptation for transmission or to sustain infection chronicity. Among this group are ESAG9 proteins, whose genes were originally identified as a component … Show more

Help me understand this report

Search citation statements

Order By: Relevance

Paper Sections

Select...
4
1

Citation Types

2
22
0

Year Published

2014
2014
2023
2023

Publication Types

Select...
4
2

Relationship

2
4

Authors

Journals

citations
Cited by 16 publications
(24 citation statements)
references
References 49 publications
2
22
0
Order By: Relevance
“…When the resulting cell line was assayed with a titration of G418, cells transfected with the NeoR gene coupled to the ESAG9 flanking sequence were killed at ≥10μg/ml G418, whereas cells transfected with the same construct but where the NeoR gene was flanked by the constitutively-expressed aldolase gene 3’UTR were viable at >750μg/ml G418 (Fig 1B). This confirmed our previous analyses demonstrating that the ESAG9 downstream sequences repress gene expression in proliferative slender forms [22]. …”
Section: Resultssupporting
confidence: 92%
See 4 more Smart Citations
“…When the resulting cell line was assayed with a titration of G418, cells transfected with the NeoR gene coupled to the ESAG9 flanking sequence were killed at ≥10μg/ml G418, whereas cells transfected with the same construct but where the NeoR gene was flanked by the constitutively-expressed aldolase gene 3’UTR were viable at >750μg/ml G418 (Fig 1B). This confirmed our previous analyses demonstrating that the ESAG9 downstream sequences repress gene expression in proliferative slender forms [22]. …”
Section: Resultssupporting
confidence: 92%
“…For ESAG9 , a previous mapping of signals in the 3’UTR that contribute to stumpy-enriched expression identified a short domain that contributed to expression in stumpy forms, but with more subtle effects in monomorphs [22]. We have confirmed regulatory control via this domain in our reporter experiments, since deletion of the element resulted in increased NeoR expression and reduced sensitivity to G418 (S2 Fig).…”
Section: Resultssupporting
confidence: 75%
See 3 more Smart Citations