The kinesin KIF1C transports APC-dependent mRNAs to cell protrusions

RNA localization and local translation are important for numerous cellular functions. In mammals, a class of mRNAs localize to cytoplasmic protrusions in an APC-dependent manner, with roles during cell migration. Here, we investigated this localization mechanism. We found that the KIF1C motor interacts with APC-dependent mRNAs and is required for their localization. Live cell imaging revealed rapid, active transport of single mRNAs over long distances that requires both microtubules and KIF1C. Two color imaging directly revealed single mRNAs transported by single KIF1C motors, with the 3’UTR being sufficient to trigger KIF1C-dependent RNA transport and localization. Moreover, KIF1C remained associated with peripheral, multimeric RNA clusters and was required for their formation. These results reveal a widespread RNA transport pathway in mammalian cells, in which the KIF1C motor has a dual role in transporting RNAs and clustering them within cytoplasmic protrusions. Interestingly, KIF1C also transports its own mRNA suggesting a possible feedback loop acting at the level of mRNA transport.

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The kinesin KIF1C transports APC-dependent mRNAs to cell protrusions

10.1101/2020.11.30.403394 ◽

2020 ◽

Author(s):

Xavier Pichon ◽

Konstadinos Moissoglu ◽

Emeline Coleno ◽

Tianhong Wang ◽

Arthur Imbert ◽

...

Keyword(s):

Cell Migration ◽

Mammalian Cells ◽

Live Cell Imaging ◽

Feedback Loop ◽

Cell Imaging ◽

Rna Localization ◽

Dependent Manner ◽

Rna Transport ◽

Cellular Functions ◽

Transport Pathway

AbstractRNA localization and local translation are important for numerous cellular functions. In mammals, a class of mRNAs localize to cytoplasmic protrusions in an APC-dependent manner, with roles during cell migration. Here, we investigated this localization mechanism. We found that the KIF1C motor interacts with APC-dependent mRNAs and is required for their localization. Live cell imaging revealed rapid, active transport of single mRNAs over long distances that requires both microtubules and KIF1C. Two color imaging directly showed single mRNAs transported by single KIF1C motors, with the 3’UTR being sufficient to trigger KIF1C-dependent RNA transport and localization. Moreover, KIF1C remained associated with peripheral, multimeric RNA clusters and was required for their formation. These results reveal an RNA transport pathway in mammalian cells, in which the KIF1C motor has a dual role both in transporting RNAs and in promoting their clustering within cytoplasmic protrusions. Interestingly, KIF1C also transports its own mRNA suggesting a possible feedback loop acting at the level of mRNA transport.

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Regulation of circular dorsal ruffles, macropinocytosis, and cell migration by RhoG and its exchange factor, Trio

Molecular Biology of the Cell ◽

10.1091/mbc.e16-06-0412 ◽

2017 ◽

Vol 28 (13) ◽

pp. 1768-1781 ◽

Cited By ~ 13

Author(s):

Alejandra Valdivia ◽

Silvia M. Goicoechea ◽

Sahezeel Awadia ◽

Ashtyn Zinn ◽

Rafael Garcia-Mata

Keyword(s):

Cell Migration ◽

Mammalian Cells ◽

Dorsal Surface ◽

Receptor Internalization ◽

Dependent Manner ◽

Cellular Functions ◽

Unique Type ◽

Exchange Factor ◽

Cellular Processes

Circular dorsal ruffles (CDRs) are actin-rich structures that form on the dorsal surface of many mammalian cells in response to growth factor stimulation. CDRs represent a unique type of structure that forms transiently and only once upon stimulation. The formation of CDRs involves a drastic rearrangement of the cytoskeleton, which is regulated by the Rho family of GTPases. So far, only Rac1 has been consistently associated with CDR formation, whereas the role of other GTPases in this process is either lacking or inconclusive. Here we show that RhoG and its exchange factor, Trio, play a role in the regulation of CDR dynamics, particularly by modulating their size. RhoG is activated by Trio downstream of PDGF in a PI3K- and Src-dependent manner. Silencing RhoG expression decreases the number of cells that form CDRs, as well as the area of the CDRs. The regulation of CDR area by RhoG is independent of Rac1 function. In addition, our results show the RhoG plays a role in the cellular functions associated with CDR formation, including macropinocytosis, receptor internalization, and cell migration. Taken together, our results reveal a novel role for RhoG in the regulation of CDRs and the cellular processes associated with their formation.

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When Yeast Cells Change their Mind: Cell Cycle 'Start' is Reversible under Starvation

10.1101/2021.10.31.466668 ◽

2021 ◽

Author(s):

Deniz Irvali ◽

Fabian P. Schlottmann ◽

Prathibha Muralidhara ◽

Iliya Nadelson ◽

N. Ezgi Wood ◽

...

Keyword(s):

Cell Cycle ◽

Mammalian Cells ◽

Live Cell Imaging ◽

Feedback Loop ◽

Cell Imaging ◽

Yeast Cells ◽

Nutrient Depletion ◽

Restriction Point ◽

Cell Cycle Inhibitor ◽

Nutrient Signaling

Eukaryotic cells decide in late G1 whether to commit to another round of genome duplication and division. This point of irreversible cell cycle commitment is a molecular switch termed 'Restriction Point' in mammals and 'Start' in budding yeast. At Start, yeast cells integrate multiple signals such as pheromones, osmolarity, and nutrients. If sufficient nutrients are lacking, cells will not pass Start. However, how the cells respond to nutrient depletion after they have made the Start decision, remains poorly understood. Here, we analyze by live cell imaging how post-Start yeast cells respond to nutrient depletion. We monitor fluorescently labelled Whi5, the cell cycle inhibitor whose export from the nucleus determines Start. Surprisingly, we find that cells that have passed Start can re-import Whi5 back into the nucleus. This occurs when cells are faced with starvation up to 20 minutes after Start. In these cells, the positive feedback loop is interrupted, Whi5 re-binds DNA, and CDK activation occurs a second time once nutrients are replenished. Cells which re-import Whi5 also become sensitive to mating pheromone again, and thus behave like pre-Start cells. In summary, we show that upon starvation the commitment decision at Start can be reversed. We therefore propose that in yeast, as has been suggested for mammalian cells, cell cycle commitment is a multi-step process, where irreversibility in face of nutrient signaling is only reached approximately 20 minutes after CDK activation at Start.

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LRRK2 mediates tubulation and vesicle sorting from membrane damaged lysosomes

10.1101/2020.01.23.917252 ◽

2020 ◽

Cited By ~ 8

Author(s):

Luis Bonet-Ponce ◽

Alexandra Beilina ◽

Chad D. Williamson ◽

Eric Lindberg ◽

Jillian H. Kluss ◽

...

Keyword(s):

Live Cell Imaging ◽

Cell Imaging ◽

Super Resolution ◽

Adaptor Protein ◽

Dependent Manner ◽

Leucine Rich Repeat ◽

Biological Functions ◽

New Process ◽

Sporadic Parkinson’S Disease

ABSTRACTMutations in the leucine rich repeat kinase 2 (LRRK2) gene are a cause of familial and sporadic Parkinson’s disease (PD). Nonetheless, the biological functions of LRRK2 remain incompletely understood. Here, we observed that LRRK2 is recruited to lysosomes that have a ruptured membrane. Using unbiased proteomics, we observed that LRRK2 is able to recruit the motor adaptor protein JIP4 to permeabilized lysosomes in a kinase-dependent manner through the phosphorylation of RAB35 and RAB10. Super-resolution live cell imaging microscopy and FIB-SEM revealed that once at the lysosomal membrane, JIP4 promotes the formation of LAMP1-negative lysosomal tubules that release membranous content from ruptured lysosomes. Released vesicular structures are able to interact with other lysosomes. Thus, we described a new process that uses lysosomal tubulation to release vesicular structures from permeabilized lysosomes. LRRK2 orchestrates this process that we name LYTL (LYsosomal Tubulation/sorting driven by LRRK2) that, given the central role of the lysosome in PD, is likely to be disease relevant.

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Integrins traffic rapidly via circular dorsal ruffles and macropinocytosis during stimulated cell migration

The Journal of Cell Biology ◽

10.1083/jcb.201007003 ◽

2011 ◽

Vol 193 (1) ◽

pp. 61-70 ◽

Cited By ~ 97

Author(s):

Zhizhan Gu ◽

Erika H. Noss ◽

Victor W. Hsu ◽

Michael B. Brenner

Keyword(s):

Functional Analysis ◽

Cell Migration ◽

Growth Factor ◽

Live Cell Imaging ◽

Cell Imaging ◽

Focal Adhesions ◽

Initial Step ◽

Ventral Surface ◽

Platelet Derived Growth Factor ◽

Trailing Edges

During cell migration, integrins are redistributed from focal adhesions undergoing disassembly at the cell’s trailing edges to new focal adhesions assembling at leading edges. The initial step of integrin redistribution is thought to require clathrin-mediated endocytosis. However, whether clathrin-mediated endocytosis functions in different contexts, such as basal versus stimulated migration, has not been determined. In this paper, we examine the spatial and temporal redistribution of integrins from focal adhesions upon stimulation by growth factors. Four-dimensional confocal live-cell imaging along with functional analysis reveals that surface integrins do not undergo significant endocytosis at ventral focal adhesions upon cell stimulation with the platelet-derived growth factor. Rather, they abruptly redistribute to dorsal circular ruffles, where they are internalized through macropinocytosis. The internalized integrins then transit through recycling endosomal compartments to repopulate newly formed focal adhesions on the ventral surface. These findings explain why integrins have long been observed to redistribute through both surface-based and internal routes and identify a new function for macropinocytosis during growth factor–induced cell migration.

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Live cell imaging analysis of the epigenetic regulation of the human endothelial cell migration at single-cell resolution

Lab on a Chip ◽

10.1039/c2lc40192d ◽

2012 ◽

Vol 12 (17) ◽

pp. 3063 ◽

Cited By ~ 12

Author(s):

Chunhong Zheng ◽

Zhilong Yu ◽

Ying Zhou ◽

Louis Tao ◽

Yuhong Pang ◽

...

Keyword(s):

Cell Migration ◽

Endothelial Cell ◽

Single Cell ◽

Epigenetic Regulation ◽

Live Cell Imaging ◽

Cell Imaging ◽

Live Cell ◽

Endothelial Cell Migration ◽

Human Endothelial Cell ◽

Imaging Analysis

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Comparative assessment of fluorescent transgene methods for quantitative imaging in human cells

Molecular Biology of the Cell ◽

10.1091/mbc.e14-06-1091 ◽

2014 ◽

Vol 25 (22) ◽

pp. 3610-3618 ◽

Cited By ~ 34

Author(s):

Robert Mahen ◽

Birgit Koch ◽

Malte Wachsmuth ◽

Antonio Z. Politi ◽

Alexis Perez-Gonzalez ◽

...

Keyword(s):

Single Molecule ◽

Protein Function ◽

Mammalian Cells ◽

Live Cell Imaging ◽

Cell Imaging ◽

Quantitative Imaging ◽

Live Cells ◽

Single Molecule Spectroscopy ◽

Mitotic Kinase ◽

Endogenous Proteins

Fluorescence tagging of proteins is a widely used tool to study protein function and dynamics in live cells. However, the extent to which different mammalian transgene methods faithfully report on the properties of endogenous proteins has not been studied comparatively. Here we use quantitative live-cell imaging and single-molecule spectroscopy to analyze how different transgene systems affect imaging of the functional properties of the mitotic kinase Aurora B. We show that the transgene method fundamentally influences level and variability of expression and can severely compromise the ability to report on endogenous binding and localization parameters, providing a guide for quantitative imaging studies in mammalian cells.

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Long-Term Live Cell Imaging of Cell Migration: Effects of Pathogenic Fungi on Human Epithelial Cell Migration

Cytoskeleton Methods and Protocols - Methods in Molecular Biology ◽

10.1007/978-1-4939-3124-8_1 ◽

2016 ◽

pp. 3-23

Author(s):

Torsten Wöllert ◽

George M. Langford

Keyword(s):

Cell Migration ◽

Epithelial Cell ◽

Live Cell Imaging ◽

Cell Imaging ◽

Pathogenic Fungi ◽

Live Cell ◽

Human Epithelial Cell ◽

Epithelial Cell Migration

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EB1 binding restricts STIM1 translocation to ER–PM junctions and regulates store-operated Ca2+ entry

The Journal of Cell Biology ◽

10.1083/jcb.201711151 ◽

2018 ◽

Vol 217 (6) ◽

pp. 2047-2058 ◽

Cited By ~ 17

Author(s):

Chi-Lun Chang ◽

Yu-Ju Chen ◽

Carlo Giovanni Quintanilla ◽

Ting-Sung Hsieh ◽

Jen Liou

Keyword(s):

Endoplasmic Reticulum ◽

Plasma Membrane ◽

Live Cell Imaging ◽

Cell Imaging ◽

Live Cell ◽

Cellular Functions ◽

Binding Ability ◽

Trapping Mechanism ◽

Spatiotemporal Regulation

The endoplasmic reticulum (ER) Ca2+ sensor STIM1 forms oligomers and translocates to ER–plasma membrane (PM) junctions to activate store-operated Ca2+ entry (SOCE) after ER Ca2+ depletion. STIM1 also interacts with EB1 and dynamically tracks microtubule (MT) plus ends. Nevertheless, the role of STIM1–EB1 interaction in regulating SOCE remains unresolved. Using live-cell imaging combined with a synthetic construct approach, we found that EB1 binding constitutes a trapping mechanism restricting STIM1 targeting to ER–PM junctions. We further showed that STIM1 oligomers retain EB1 binding ability in ER Ca2+-depleted cells. By trapping STIM1 molecules at dynamic contacts between the ER and MT plus ends, EB1 binding delayed STIM1 translocation to ER–PM junctions during ER Ca2+ depletion and prevented excess SOCE and ER Ca2+ overload. Our study suggests that STIM1–EB1 interaction shapes the kinetics and amplitude of local SOCE in cellular regions with growing MTs and contributes to spatiotemporal regulation of Ca2+ signaling crucial for cellular functions and homeostasis.

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