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4 research outputs found

Blocking late stages of splicing quickly limits pre-spliceosome assembly in vivo

Author: Gonzalo I. Mendoza-Ochoa
Isabella E. Maudlin
J. David Barrass
Jean D. Beggs
Longtine M
Mendoza-Ochoa GI
Noble SM
Publication venue: 'Informa UK Limited'
Publication date: 04/09/2019
Field of study

Crossref

Edinburgh Research Explorer

Tuning degradation to achieve specific and efficient protein depletion

Author: Barrass J David
Beggs Jean D
Maudlin Isabella E
Mendoza-Ochoa Gonzalo I
Sani Emanuela
Publication venue: 'MyJove Corporation'
Publication date: 20/07/2019
Field of study

Crossref

Edinburgh Research Explorer

PREditOR: A synthetic biology approach to removing heterochromatin from cells

Author: A Losada
AH Peters
AJ Bannister
AJ Bannister
AM Ainsztein
AM Olszak
B Koch
BA Sullivan
C Obuse
D Gerlich
DL Bodor
HD Folco
IM Krouwels
Isabella E. Maudlin
JC Peng
JH Bergmann
K Ekwall
K Jaqaman
L Chu
L Chu
LL Sullivan
M Carmena
M Gartenberg
M Melcher
M Nakano
Mar Carmena
ME Aldrup-Macdonald
N Nonaka
N Saksouk
NM Martins
O Molina
Oscar Molina
P Bernard
P Oberdoerffer
R Cao
RB Slee
RC Allshire
RJ Sims 3rd
S Cardinale
S Haldar
S Rea
SA Ribeiro
SS Levine
T Fukagawa
T Hirota
W Fischle
WC Earnshaw
William C. Earnshaw
X Liu
Y Yamagishi
Y Yamagishi
Publication venue: 'Springer Science and Business Media LLC'
Publication date: 01/01/2016
Field of study

It is widely accepted that heterochromatin is necessary to maintain genomic stability. However, direct experimental evidence supporting this is slim. Previous studies using either enzyme inhibitors, gene knockout or knockdown studies all are subject to the caveat that drugs may have off-target effects and enzymes that modify chromatin proteins to support heterochromatin formation may also have numerous other cellular targets as well. Here, we describe PREditOR (protein reading and editing of residues), a synthetic biology approach that allows us to directly remove heterochromatin from cells without either drugs or global interference with gene function. We find that removal of heterochromatin perturbs mitotic progression and causes a dramatic increase in chromosome segregation defects, possibly as a result of interfering with the normal centromeric localization of the chromosomal passenger complex. ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (doi:10.1007/s10577-016-9539-3) contains supplementary material, which is available to authorized users

Crossref

Springer - Publisher Connector

PubMed Central

Edinburgh Research Explorer

VSG mRNA levels are regulated by the production of functional VSG protein.

Author: Carrington Mark
Kelly Steve
Maudlin Isabella E
Schwede Angela
Publication venue: Mol Biochem Parasitol
Publication date: 19/12/2020
Field of study

The bloodstream form of Trypanosoma brucei persists in mammalian hosts through a population survival strategy depending on antigenic variation of a cell surface coat composed of the variant surface glycoprotein (VSG). The integrity of the VSG coat is essential and blocking its synthesis results in a cell division cycle arrest just prior to cytokinesis. This observation indicates that VSG levels are monitored and that the cell has mechanisms to respond to a disruption of synthesis. Here, the regulation of VSG mRNA levels has been investigated by first measuring VSG mRNA copy number, and second using ectopic expression of VSG transgenes containing premature termination codons. The findings are that (i) VSG mRNA copy number varies with the identity of the VSG and (ii) a pathway detects synthesis of non-functional VSG protein and results in an increase in VSG mRNA levels

Oxford University Research Archive

Apollo (Cambridge)