Copy Link
Add to Bookmark
Report

dictyNews Volume 32 Number 03

eZine's profile picture
Published in 
Dicty News
 · 10 months ago

dictyNews 
Electronic Edition
Volume 32, number 3
January 30, 2009

Please submit abstracts of your papers as soon as they have been
accepted for publication by sending them to dicty@northwestern.edu
or by using the form at
http://dictybase.org/db/cgi-bin/dictyBase/abstract_submit.

Back issues of dictyNews, the Dicty Reference database and other
useful information is available at dictyBase - http://dictybase.org.

=========
Abstracts
=========



The 3-Dimensional Dynamics of Actin Waves,
a Model of Cytoskeletal Self-organization

Till Bretschneider1, 3,§, Kurt Anderson2, 5,§, Mary Ecke1,
Annette Mueller-Taubenberger1, 4,  Britta Schroth-Diez2, 
Hellen C. Ishikawa-Ankerhold1, and Guenther Gerisch1*

1 Max-Planck-Institut fuer Biochemie, Am Klopferspitz 18,
D-82152 Martinsried, Germany.
2 Max-Planck-Institut fuer molekulare Zellbiologie und Genetik,
Pfotenhauerstrasse 108, D 01307 Dresden, Germany.
3 Present address: Warwick Systems Biology, Coventry House,
University of Warwick, Coventry CV4 7AL, UK.
4 Present address: Adolf Butenandt Institute / Cell Biology and Munich
Center for Integrated Protein Science (CIPSM), Ludwig Maximilians Universitaet,
Schillerstrasse 42, D-80336 Muenchen, Germany.
5 Present address: Leader Light Microscopy, Beatson Institute for Cancer
Research, Garscube Estate, Switchback Road, Glasgow, G61 1BD, Scotland UK.
§ These two authors contributed equally to the work.

*Correspondence should be addressed to Dr. Guenther Gerisch,
Max-Planck-Institut fuer Biochemie, D-82152 Martinsried, Germany.  
phone: (+49) 89-8578-2326; fax: (+49) 89-8578-3885;  
e-mail: gerisch@biochem.mpg.de


Biophys.J., in press.
   
Actin polymerization is typically initiated at specific sites in a
cell by membrane-bound protein complexes, and the resulting structures 
are involved in specialized cellular functions, such as migration, 
particle uptake, or mitotic division. Here we analyze the potential 
of the actin system to self-organize into waves that propagate on 
the planar, substrate-attached membrane of a cell. We show that 
self-assembly involves the ordered recruitment of proteins from 
the cytoplasmic pool, and relate the organization of actin waves 
to their capacity for applying force. Three proteins are shown to 
form distinct 3-dimensional patterns in the actin waves. Myosin-IB 
is enriched at the wave front and close to the plasma membrane, 
the Arp2/3 complex is distributed throughout the waves, and 
coronin forms a sloping layer on top of them. CARMIL, a protein 
that links myosin-IB to the Arp2/3 complex, is also recruited to
the waves. Wave formation does not depend on signals transmitted 
by heterotrimeric G-proteins, nor does their propagation require 
SCAR, a regulator upstream of the Arp2/3 complex. Propagation 
of the waves is based on an actin treadmilling mechanism,
indicating a program that couples actin assembly to disassembly 
in a 3-dimensional pattern. When waves impinge on the cell 
perimeter, they push the edge forward, when they reverse direction, 
the cell border is paralyzed. These data show that force-generating, 
highly organized supramolecular networks are autonomously 
formed in live cells from molecular motors and proteins
controlling actin polymerization and depolymerization.


Submitted by: Guenther Gerisch [gerisch@biochem.mpg.de]
--------------------------------------------------------------------------------


A measure of endosomal pH by flow cytometry in Dictyostelium

Anna Marchetti, Emmanuelle Lelong and Pierre Cosson

BMC Research Notes 2009, 2:7

Dictyostelium amoebae are frequently used to study the organization 
and function of the endocytic pathway, and specific protocols are 
essential to measure the dynamics of endocytic compartments and 
their internal pH. We have revisited these classical protocols to
measure more accurately endosomal pH, making use of a fluorescent
probe (Oregon green) more adequate for very acidic pH values. This 
pH-sensitive probe was combined with a pH-insensitive marker, 
in order to visualize simultaneously endosome dynamics and pH 
changes. Finally, a flow cytometer was used to measure endosomal 
pH in individual cells. Using these simple protocols the endosomal
pH of endocytic compartments can be assessed accurately, revealing
the extreme acidity of Dictyostelium lysosomes (pH <3.5).


Submitted by: Emmanuelle Lelong [emmanuelle.lelong@unige.ch]
==============================================================
[End dictyNews, volume 32, number 3]

← previous
next →
loading
sending ...
New to Neperos ? Sign Up for free
download Neperos App from Google Play
install Neperos as PWA

Let's discover also

Recent Articles

Recent Comments

Neperos cookies
This website uses cookies to store your preferences and improve the service. Cookies authorization will allow me and / or my partners to process personal data such as browsing behaviour.

By pressing OK you agree to the Terms of Service and acknowledge the Privacy Policy

By pressing REJECT you will be able to continue to use Neperos (like read articles or write comments) but some important cookies will not be set. This may affect certain features and functions of the platform.
OK
REJECT