dictyNews
Electronic Edition
Volume 38, number 4
February 3, 2012

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Abstracts
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Evolution of self-organisation in Dictyostelia by adaptation of a 
non-selective phosphodiesterase and a matrix component for 
regulated cAMP degradation

Yoshinori Kawabe, Karin E. Weening, Jacques Marquay-Markiewicz 
and Pauline Schaap*

College of Life Sciences, University of Dundee, Dundee DD15EH, UK


Development, in press

Dictyostelium discoideum amoebas coordinate aggregation and 
morphogenesis by secreting cAMP pulses that propagate as waves 
through fields of cells and multicellular structures. To retrace how this 
mechanism for self-organisation evolved, we studied the origin of the 
cAMP phosphodiesterase PdsA and its inhibitor PdiA, which are 
essential for cAMP wave propagation. D.discoideum and other species 
that use cAMP to aggregate reside in group 4 of the four major groups 
of Dictyostelia. We found that groups 1-3 express a non-specific, low 
affinity ortholog of PdsA, which gained cAMP selectivity and increased 
200-fold in affinity in group 4. A low affinity group 3 PdsA only partially 
restored aggregation of a D.discoideum pdsA null mutant, but was more 
effective at restoring fruiting body morphogenesis. Deletion of a group 2 
PdsA gene resulted in disruption of fruiting body morphogenesis, but 
left aggregation unaffected. Together, these results show that groups 
1-3 use a low affinity PdsA for morphogenesis that is neither suited 
nor required for aggregation. PdiA belongs to a family of matrix proteins 
that are present in all Dictyostelia and consist mainly of cysteine-rich 
repeats. However, in its current form with several extensively modified 
repeats, PdiA is only present in the group 4. PdiA is essential for 
initiating spiral cAMP waves, which, by organizing large territories, 
generate the large fruiting structures that characterize group 4. We 
conclude that efficient cAMP-mediated aggregation in group 4 evolved 
by recruitment and adaptation of a non-selective phosphodiesterase 
and a matrix component into a system for regulated cAMP 
degradation.


Submitted by Pauline Schaap [[log in to unmask]]
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Regulation of aggregate size and pattern by adenosine and caffeine 
in cellular slime molds.

Jaiswal P, Soldati T, Thewes S, Baskar R.


BMC Dev Biol. 2012 Jan 23;12(1):5.
 
BACKGROUND: Multicellularity in cellular slime molds is achieved 
by aggregation of several hundreds to thousands of cells. In the model 
slime mold Dictyostelium discoideum, adenosine is known to increase 
the aggregate size and its antagonist caffeine reduces the aggregate 
size. However, it is not clear if the actions of adenosine and caffeine 
are evolutionarily conserved among other slime molds known to use 
structurally unrelated chemoattractants.
 
RESULTS: We have examined how the known factors affecting 
aggregate size are modulated by adenosine and caffeine. Result: 
Adenosine and caffeine induced the formation of large and small 
aggregates respectively, in evolutionarily distinct slime molds known 
to use diverse chemoattractants for their aggregation. Due to its 
genetic tractability, we chose D. discoideum to further investigate the 
factors affecting aggregate size. The changes in aggregate size are 
caused by the effect of the compounds on several parameters such 
as cell number and size, cell-cell adhesion, cAMP signal relay and 
cell counting mechanisms. While some of the effects of these two 
compounds are opposite to each other, interestingly, both 
compounds increase the intracellular glucose level and strengthen 
cell-cell adhesion. These compounds also inhibit the synthesis of 
cAMP phosphodiesterase (PdsA), weakening the relay of extracellular 
cAMP signal. Adenosine as well as caffeine rescue mutants impaired 
in stream formation (pde4- and pdiA-) and colony size (smlA- and ctnA-) 
and restore their parental aggregate size.
 
CONCLUSION: Adenosine increased the cell division timings thereby 
making large number of cells available for aggregation and also it 
marginally increased the cell size contributing to large aggregate size. 
Reduced cell division rates and decreased cell size in the presence of 
caffeine makes the aggregates smaller than controls. Both the 
compounds altered the speed of the chemotactic amoebae causing 
a variation in aggregate size. Our data strongly suggests that cytosolic 
glucose and extracellular cAMP levels are the other major determinants 
regulating aggregate size and pattern. Importantly, the aggregation 
process is conserved among different lineages of cellular slime molds 
despite using unrelated signalling molecules for aggregation.


Submitted by R. Baskar [[log in to unmask]]
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ZizB, a novel RacGEF regulates development, cell motility and 
cytokinesis in Dictyostelium

Nicholl K. Pakes*, Douwe Veltman*, Francisco Rivero, Jamal Nasir, 
Robert Insall, and Robin S.B. Williams


J. Cell Sci., in press

Dock (Dedicator of Cytokinesis) proteins represent a family of Guanine 
nucleotide Exchange Factors (GEFs) that include the well studied Dock180 
family and the poorly characterised zizimin family. Our current understanding 
of Dock180 function is to regulate Rho small GTPases, playing a role in a 
number of cell processes including cell migration, development and division. 
Here, we have employed a tractable model for cell motility research, 
Dictyostelium discoideum, to help elucidate the role of the related zizimin 
proteins. We show that gene ablation of zizA causes no change in 
development whereas ablation of zizB gives rise to an aberrant 
developmental morphology and a reduction in cell directionality and velocity, 
and altered cell shape. Fluorescently labeled ZizA protein associates with 
the microtubule organizing centre (MTOC), whereas the ZizB protein 
exhibits cortical enrichment. Overexpression of ZizB also causes an 
increase in the number filopodia and a partial inhibition of cytokinesis. 
Analysis of ZizB protein binding partners indicates a direct binding to Rac1a 
and a range of actin-interacting proteins. In conclusion our work provides 
the first insight into the molecular and cellular functions of zizimin GEF 
proteins playing a role in cell movement, filopodia formation and cytokinesis.


Submitted by  Robin Williams [[log in to unmask]]
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[End dictyNews, volume 38, number 4]