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64 research outputs found

A novel di-acidic motif facilitates ER export of the syntaxin SYP31

Author: Brandizzi Federica
Chatre Laurent
Maneta-Peyret Lilly
Melser Su
Moreau Patrick
Wattelet-Boyer Valérie
Publication venue: Oxford University Press
Publication date: 01/01/2009
Field of study

It is generally accepted that ER protein export is largely influenced by the transmembrane domain (TMD). The situation is unclear for membrane-anchored proteins such as SNAREs, which are anchored to the membrane by their TMD at the C-terminus. For example, in plants, Sec22 and SYP31 (a yeast Sed5 homologue) have a 17 aa TMD but different locations (ER/Golgi and Golgi), indicating that TMD length alone is not sufficient to explain their targeting. To establish the identity of factors that influence SNARE targeting, mutagenesis and live cell imaging experiments were performed on SYP31. It was found that deletion of the entire N-terminus domain of SYP31 blocked the protein in the ER. Several deletion mutants of different parts of this N-terminus domain indicated that a region between the SNARE helices Hb and Hc is required for Golgi targeting. In this region, replacement of the aa sequence MELAD by GAGAG or MALAG retained the protein in the ER, suggesting that MELAD may function as a di-acidic ER export motif EXXD. This suggestion was further verified by replacing the established di-acidic ER export motif DLE of a type II Golgi protein AtCASP and a membrane-anchored type I chimaera, TMcCCASP, by MELAD or GAGAG. The MELAD motif allowed the proteins to reach the Golgi, whereas the motif GAGAG was found to be insufficient to facilitate ER protein export. Our analyses indicate that we have identified a novel and transplantable di-acidic motif that facilitates ER export of SYP31 and may function for type I and type II proteins in plants

CiteSeerX

PubMed Central

Efficient mitochondrial targeting relies on co-operation of multiple protein signals in plants

Author: Addya
Alder
Andrew S. Jack
Bannai
Batoko
Boevink
Brandizzi
Brink
Chabregas
Christensen
daSilva
Duby
Federica Brandizzi
Garcia
Gaume
Gavel
Glaser
Guda
Hammen
Haseloff
Heard
Hoffman
Hofmann
Hulo
Kleinberger-Doron
Krogh
Laurent Chatre
Lee
Lemire
Letunic
Logan
Loren A. Matheson
Ma
Martin
Matouschek
Millar
Nagai
Neupert
Nielsen
Oikawa
Pujol
Roise
Sally L. Hanton
Sambrook
Schatz
Schultz
Small
Sunderland
Yano
Young
Publication venue: Oxford University Press
Publication date
Field of study

To date, the most prevalent model for transport of pre-proteins to plant mitochondria is based on the activity of an N-terminal extension serving as a targeting peptide. Whether the efficient delivery of proteins to mitochondria is based exclusively on the action of the N-terminal extension or also on that of other protein determinants has yet to be defined. A novel mechanism is reported here for the targeting of a plant protein, named MITS1, to mitochondria. It was found that MITS1 contains an N-terminal extension that is responsible for mitochondrial targeting. Functional dissection of this extension shows the existence of a cryptic signal for protein targeting to the secretory pathway. The first 11 amino acids of the N-terminal extension are necessary to overcome the activity of this signal sequence and target the protein to the mitochondria. These data suggest that co-operation of multiple determinants within the N-terminal extension of mitochondrial proteins may be necessary for efficient mitochondrial targeting. It was also established that the presence of a tryptophan residue toward the C-terminus of the protein is crucial for mitochondrial targeting, as mutation of this residue results in a redistribution of MITS1 to the endoplasmic reticulum and Golgi apparatus. These data suggest a novel targeting model whereby protein traffic to plant mitochondria is influenced by domains in the full-length protein as well as the N-terminal extension

Crossref

PubMed Central

Nuclear Mitochondrial DNA Activates Replication in Saccharomyces cerevisiae

Author: AJ van Brabant
AM Breier
B Amati
BC Hyman
BC Hyman
BJ Brewer
C Noutsos
C Sacerdot
C Santocanale
C Turner
CA Nieduszynski
CA Nieduszynski
David Kirkpatrick
DM Becker
DM MacAlpine
DT Stinchcomb
E Goldin
E Richly
F Srienc
GE Crooks
H Blanc
H Blanc
H Fukuhara
H Tourriere
HI Hadler
HJ McCune
J Hindley
JA Huberman
JE Willett-Brozick
JF Theis
JJ Donato
JJ Wyrick
JP Vartanian
JR Broach
JV Van Houten
JW Shay
K Borensztajn
K Struhl
L Crabbe
L Margulys
Laurent Chatre
M Podnar
M Ricchetti
M Ricchetti
M Ricchetti
M Zuker
Miria Ricchetti
MK Raghuraman
PC Angeletti
RA Reid
RS Sikorski
S Lenglez
S Lin
SS Walker
TD Schneider
W Feng
W Xu
X Yu
Y Marahrens
Publication venue: Public Library of Science
Publication date: 01/01/2010
Field of study

The nuclear genome of eukaryotes is colonized by DNA fragments of mitochondrial origin, called NUMTs. These insertions have been associated with a variety of germ-line diseases in humans. The significance of this uptake of potentially dangerous sequences into the nuclear genome is unclear. Here we provide functional evidence that sequences of mitochondrial origin promote nuclear DNA replication in Saccharomyces cerevisiae. We show that NUMTs are rich in key autonomously replicating sequence (ARS) consensus motifs, whose mutation results in the reduction or loss of DNA replication activity. Furthermore, 2D-gel analysis of the mrc1 mutant exposed to hydroxyurea shows that several NUMTs function as late chromosomal origins. We also show that NUMTs located close to or within ARS provide key sequence elements for replication. Thus NUMTs can act as independent origins, when inserted in an appropriate genomic context or affect the efficiency of pre-existing origins. These findings show that migratory mitochondrial DNAs can impact on the replication of the nuclear region they are inserted in

CiteSeerX

Public Library of Science (PLOS)

Crossref

PubMed Central