162,578 research outputs found
Sensor potency of the moonlighting enzyme-decorated cytoskeleton
Background: There is extensive evidence for the interaction of metabolic enzymes with the eukaryotic
cytoskeleton. The significance of these interactions is far from clear.
Presentation of the hypothesis: In the cytoskeletal integrative sensor hypothesis presented here, the cytoskeleton
senses and integrates the general metabolic activity of the cell. This activity depends on the binding to the
cytoskeleton of enzymes and, depending on the nature of the enzyme, this binding may occur if the enzyme is
either active or inactive but not both. This enzyme-binding is further proposed to stabilize microtubules and
microfilaments and to alter rates of GTP and ATP hydrolysis and their levels.
Testing the hypothesis: Evidence consistent with the cytoskeletal integrative sensor hypothesis is presented in the
case of glycolysis. Several testable predictions are made. There should be a relationship between post-translational
modifications of tubulin and of actin and their interaction with metabolic enzymes. Different conditions of cytoskeletal
dynamics and enzyme-cytoskeleton binding should reveal significant differences in local and perhaps global levels and
ratios of ATP and GTP. The different functions of moonlighting enzymes should depend on cytoskeletal binding.
Implications of the hypothesis: The physical and chemical effects arising from metabolic sensing by the cytoskeleton
would have major consequences on cell shape, dynamics and cell cycle progression. The hypothesis provides a
framework that helps the significance of the enzyme-decorated cytoskeleton be determined
Synthesis of spectrin in avian erythroid cells: association of nascent polypeptide chains with the cytoskeleton
The site of synthesis of spectrin was investigated in erythroid cells from 10-day chicken embryos. After various periods of [35S]methionine incorporation the cells were lysed in a Triton X-100 (TX-100)-containing buffer and were separated into a TX-100-soluble and -insoluble (cytoskeletal) fraction. Analysis of these two fractions by two-dimensional gel electrophoresis after a short pulse-labeling period reveals that alpha-spectrin nascent polypeptides are present predominantly in the TX-100-insoluble fraction. These polypeptides can be immunoprecipitated with alpha-spectrin antisera and the [35S]methionine incorporated into them during a short pulse can be chased into mature alpha-spectrin molecules. The alpha-spectrin nascent polypeptide chains are released quantitatively from the TX-100 cytoskeleton by treatment of lysed cells with puromycin, suggesting that they themselves are not associated with the cytoskeleton. A small fraction of the newly synthesized mature alpha-spectrin molecules is rapidly incorporated into the cytoskeleton, as shown by the fact that they are not released by the puromycin treatment; the rest are recovered in the soluble fraction. These results suggest that alpha-spectrin is synthesized in association with the cytoskeleton during chicken erythropoiesis and assembles onto the membrane-cytoskeleton posttranslationally
Cytoskeleton and Cell Motility
The present article is an invited contribution to the Encyclopedia of
Complexity and System Science, Robert A. Meyers Ed., Springer New York (2009).
It is a review of the biophysical mechanisms that underly cell motility. It
mainly focuses on the eukaryotic cytoskeleton and cell-motility mechanisms.
Bacterial motility as well as the composition of the prokaryotic cytoskeleton
is only briefly mentioned. The article is organized as follows. In Section III,
I first present an overview of the diversity of cellular motility mechanisms,
which might at first glance be categorized into two different types of
behaviors, namely "swimming" and "crawling". Intracellular transport, mitosis -
or cell division - as well as other extensions of cell motility that rely on
the same essential machinery are briefly sketched. In Section IV, I introduce
the molecular machinery that underlies cell motility - the cytoskeleton - as
well as its interactions with the external environment of the cell and its main
regulatory pathways. Sections IV D to IV F are more detailed in their
biochemical presentations; readers primarily interested in the theoretical
modeling of cell motility might want to skip these sections in a first reading.
I then describe the motility mechanisms that rely essentially on
polymerization-depolymerization dynamics of cytoskeleton filaments in Section
V, and the ones that rely essentially on the activity of motor proteins in
Section VI. Finally, Section VII is devoted to the description of the
integrated approaches that have been developed recently to try to understand
the cooperative phenomena that underly self-organization of the cell
cytoskeleton as a whole.Comment: 31 pages, 16 figures, 295 reference
Models of dynamic extraction of lipid tethers from cell membranes
When a ligand that is bound to an integral membrane receptor is pulled, the
membrane and the underlying cytoskeleton can deform before either the membrane
delaminates from the cytoskeleton or the ligand detaches from the receptor. If
the membrane delaminates from the cytoskeleton, it may be further extruded and
form a membrane tether. We develop a phenomenological model for this processes
by assuming that deformations obey Hooke's law up to a critical force at which
the cell membrane locally detaches from the cytoskeleton and a membrane tether
forms. We compute the probability of tether formation and show that they can be
extruded only within an intermediate range of force loading rates and pulling
velocities. The mean tether length that arises at the moment of ligand
detachment is computed as are the force loading rates and pulling velocities
that yield the longest tethers.Comment: 16 pages, 7 figure
Actin cytoskeleton-dependent regulation of corticotropin-releasing factor receptor heteromers
Stress responses are highly nuanced and variable, but how this diversity is achieved by modulating receptor function is largely unknown. Corticotropin-releasing factor receptors (CRFRs), class B G protein–coupled receptors, are pivotal in mediating stress responses. Here we show that the two known CRFRs interact to form heteromeric complexes in HEK293 cells coexpressing both CRFRs and in vivo in mouse pancreas. Coimmunoprecipitation and mass spectrometry confirmed the presence of both CRF1R and CRF2βR, along with actin in these heteromeric complexes. Inhibition of actin filament polymerization prevented the transport of CRF2βR to the cell surface but had no effect on CRF1R. Transport of CRF1R when coexpressed with CRF2βR became actin dependent. Simultaneous stimulation of cells coexpressing CRF1R+CRF2βR with their respective high-affinity agonists, CRF+urocortin2, resulted in approximately twofold increases in peak Ca2+responses, whereas stimulation with urocortin1 that binds both receptors with 10-fold higher affinity did not. The ability of CRFRs to form heteromeric complexes in association with regulatory proteins is one mechanism to achieve diverse and nuanced function
cis-acting sequences and trans-acting factors in the localization of mRNA for mitochondrial ribosomal proteins
mRNA localization is a conserved post-transcriptional process crucial for a variety of systems. Although several mechanisms have been identified, emerging evidence suggests that most transcripts reach the protein functional site by moving along cytoskeleton elements. We demonstrated previously that mRNA for mitochondrial ribosomal proteins are asymmetrically distributed in the cytoplasm, and that localization in the proximity of mitochondria is mediated by the 3′-UTR. Here we show by biochemical analysis that these mRNA transcripts are associated with the cytoskeleton through the microtubule network. Cytoskeleton association is functional for their intracellular localization near the mitochondrion, and the 3′-UTR is involved in this cytoskeleton-dependent localization. To identify the minimal elements required for localization, we generated DNA constructs containing, downstream from the GFP gene, deletion mutants of mitochondrial ribosomal protein S12 3′-UTR, and expressed them in HeLa cells. RT-PCR analysis showed that the localization signals responsible for mRNA localization are located in the first 154 nucleotides. RNA pulldown assays, mass spectrometry, and RNP immunoprecipitation assay experiments, demonstrated that mitochondrial ribosomal protein S12 3′-UTR interacts specifically with TRAP1 (tumor necrosis factor receptor-associated protein1), hnRNPM4 (heterogeneous nuclear ribonucleoprotein M4), Hsp70 and Hsp60 (heat shock proteins 70 and 60), and α-tubulin in vitro and in vivo
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