The Role of Chloride Channels in Regulation of Pulmonary Artery Smooth Muscle Cell Proliferation

Liang, Wenbin

19 November 2013

Pulmonary arterial hypertension (PAH) is a rare but fatal disease with an annual mortality rate of 15% despite current therapies. Uncontrolled proliferation of pulmonary artery smooth muscle cells (PASMCs) results in adverse vascular remodeling contributing to PAH. Understanding the mechanisms of PASMC proliferation may identify new targets for treatment. Chloride currents/channels (ICl) are expressed in PASMCs and their roles in proliferation have been suggested based on their importance in resting membrane potential and cell volume regulation. The present study explored the role of ICl in proliferation in rat and human PASMCs. We found that either nonspecific ICl inhibitors (DIDS or NPPB) or a putative specific blocker of swelling-activated ICl (ICl,swell) reduced proliferation of PASMCs cultured in serum-containing media. Patch-clamp studies showed that proliferating PASMCs had increased baseline ICl and ICl,swell in association with depolarized membrane potentials. Quantitative real-time RT-PCR studies identified expressions of CLC-3, a candidate gene of ICl,swell, and several other CLC genes in proliferating PASMCs. While selective knockdown of CLC-3 with lentiviral shRNA reduced PASMC proliferation, it had no effect on ICl,swell. These findings are consistent with the conclusion that ICl regulate proliferation of PASMCs and suggest that selective ICl inhibition may be useful in treating pulmonary arterial hypertension.

Pulmonary arterial hypertension

Pulmonary artery smooth muscle cell

Proliferation

Chloride channel

Cell volume

Membrane potential

RNA interference

Lentivirus

CLC channels

CLC-3

DIDS

DCPIB

0719

Marcadores fenot?picos para caracteriza??o de caprinos com diferentes n?veis de resist?ncia ?s endoparasitoses gastrintestinais / Phenotypic markers to characterizeE goats with different levels of resistance to gastrointestinal nematodes

Coutinho, Renata Maria Alves

28 February 2012

Made available in DSpace on 2014-12-17T15:34:44Z (GMT). No. of bitstreams: 1 RenataMAC_DISSERT.pdf: 1125273 bytes, checksum: 6bd33833f33ca21674933995a1ccf14a (MD5) Previous issue date: 2012-02-28 / Coordena??o de Aperfei?oamento de Pessoal de N?vel Superior / The aim of this study was to evaluate and characterize phenotypically goats with different levels of resistance to gastrointestinal nematodes. For a period of 93 days, 60 F2 goats originated from ? Saanen and ? Anglo- nubian animals were kept in the same area of pasture. Every seven days, feces and blood were collected for eggs per gram counts of feces (EPG) and cultures of feces and to determinate the number of eosinophils, packed cell volume and total plasma protein, respectively. On the same day, the animals were weighed and submitted to body score condition and FAMACHA method to worm control. Based on the average of EPG, the twelve animals with the highest average (susceptible group) and the twelve animals with the lowest average of EPG (resistant group) were selected, slaughtered and necropsied to recovery, counting andparasites identification. The resistant animals present lower EPG mean (P <0.0001) and 4.7 folder less parasites than susceptible animals. The resistant group presented higher mean packed cell volume (26.48%) and total plasma protein (6.24 g / dl) than susceptible one (24,04% e 5,82g/dl, respectively). The average number of eosinophils was similar in both groups The Haemonchus sp. was the most prevalent in the culture of feces, followed by Trischostrongylus sp. and Oesophagostomum sp.. The counting of nematodes in the abomasum of susceptible group was higher than in resistant one. The species identified were H. contortus in abomasums and T. colubriformis in small intestine. It can be concluded that EPG, packed cell volume and total plasma protein were useful phenotypic markers to identify animals as resistant and susceptible to gastrointestinal nematodes infections / O presente trabalho teve como objetivo de avaliar e caracterizar fenotipicamente caprinos com diferentes n?veis de resist?ncia a nematoides gastrintestinais. Em um per?odo de 93 dias, 60 caprinos F2 oriundos do cruzamento de animais ? Saanen e ? Anglo-nubiano foram mantidos em uma mesma ?rea de pastagem cultivada irrigada de capim Tanz?nia (Panicum maximum Jacq. Cv Tanz?nia). A cada sete dias, fezes e sangue foram coletados para contagem de ovos por grama de fezes (OPG), coproculturas, contagem de eosin?filos, determina??o de volume globular e prote?na plasm?tica total, respectivamente. No mesmo dia das coletas, os animais foram pesados e avaliados quanto ao escore da condi??o corporal e grau de anemia com aux?lio no cart?o FAMACHA. Com base na m?dia de OPG, os doze animais com as maiores m?dias de OPG (grupo suscept?vel) e os doze animais com as menores m?dias de OPG (grupo resistente) foram identificados e selecionados para serem abatidos e necropsiados para a recupera??o, contagem e identifica??o dos parasitos presentes. Os animais pertencentes ao grupo resistente apresentaram menor m?dia de OPG (P<0,0001) e 4,7 vezes menos parasitos adultos do que os animais do grupo suscept?vel. O grupo resistente obteve maior m?dia de volume globular (26,48%) e prote?na plasm?tica total (6,24 g/dl) do que os animais suscept?veis (24,04% e 5,82g/dl, respectivamente). A m?dia de eosin?filos foi semelhante nos dois grupos .O g?nero Haemonchus foi o mais prevalente a nas coproculturas, seguido por Trischostrongylus e Oesophagostomum. A contagem de nematoides foi maior no abomaso do grupo suscept?vel do que no grupo resistente. As esp?cies identificadas foram H. contortus no abomaso e T. colubriformis no intestino delgado. Conclui-se que OPG, volume globular e prote?na plasm?tica total foram marcadores fenot?picos eficientes para identificar animais resistentes e suscept?veis ?s infec??es causadas por nematoides gastrintestinais

Caprinos

FAMACHA

Nematoides

OPG

Resist?ncia

Volume globular

Goats

EPG

FAMACHA

Nematode

Packed cell volume

Resistance

Relação entre o volume da célula e dinâmica do ciclo celular em mamíferos

Magno, Alessandra Cristina Gomes

22 March 2016

Submitted by Renata Lopes (renatasil82@gmail.com) on 2017-05-31T15:25:44Z No. of bitstreams: 1 alessandracristinagomesmagno.pdf: 3807060 bytes, checksum: a3775aee860af7ea06cde6b9d587ab80 (MD5) / Rejected by Adriana Oliveira (adriana.oliveira@ufjf.edu.br), reason: on 2017-06-01T11:41:14Z (GMT) / Submitted by Renata Lopes (renatasil82@gmail.com) on 2017-06-01T11:44:40Z No. of bitstreams: 1 alessandracristinagomesmagno.pdf: 3807060 bytes, checksum: a3775aee860af7ea06cde6b9d587ab80 (MD5) / Approved for entry into archive by Adriana Oliveira (adriana.oliveira@ufjf.edu.br) on 2017-06-01T11:47:06Z (GMT) No. of bitstreams: 1 alessandracristinagomesmagno.pdf: 3807060 bytes, checksum: a3775aee860af7ea06cde6b9d587ab80 (MD5) / Made available in DSpace on 2017-06-01T11:47:06Z (GMT). No. of bitstreams: 1 alessandracristinagomesmagno.pdf: 3807060 bytes, checksum: a3775aee860af7ea06cde6b9d587ab80 (MD5) Previous issue date: 2016-03-22 / O objetivo principal deste trabalho é adicionar e analisar uma equação que repre senta o volume no modelo dinâmico do ciclo celular de mamíferos proposto por Gérard e Goldbeter (2011). A divisão celular ocorre quando o complexo ciclinaB/Cdk1(quínase dependente de ciclina) é totalmente degradado atingindo um valor mínimo. Neste ponto, a célula é divida em duas novas células filhas e cada uma irá conter a metade do conteúdo citoplasmático da célula mãe. As equações do modelo de base são válidas apenas se o volume celular, onde as reações ocorrem, é constante. Quando o volume celular não é constante, isto é, a taxa de variação do volume em relação ao tempo é explicitamente levada em consideração no modelo matemático, então as equações do modelo original não são mais válidas. Portanto, todas as equações foram modificadas a partir do princípio de conservação das massas para considerar um volume que varia ao longo do tempo. Por meio desta abordagem, o volume celular afeta todas as variáveis do modelo. Dois méto dos diferentes de simulação foram efetuados: determinista e estocástico. Na simulação estocástica, o volume afeta todos os parâmetros do modelo que possuem de alguma forma unidade molar, enquanto que no determinista, ele é incorporado nas equações diferen ciais. Na simulação determinista, as espécies bioquímicas podem estar em unidades de concentração, enquanto na simulação estocástica tais espécies devem ser convertidas para número de moléculas que são diretamente proporcional ao volume celular. Em um esforço para entender a influência da nova equação sobre o modelo uma análise de estabilidade foi feita. Isso esclarece como o novo parâmetro µ, fator de crescimento do volume celular, impacta na estabilidade do ciclo limite do modelo. Para encontrar a solução aproximada do modelo determinista, o método Runge Kutta de quarta ordem foi implementado. Já para o modelo estocástico, o método direto de Gillespie foi usado. Para concluir, um modelo mais preciso, em comparação ao modelo de base, foi desenvolvido ao levar em consideração a influência da taxa de variação do volume celular sobre o ciclo celular. / The main goal of this work is to add and analyse an equation that represents the volume in a dynamical model of the mammalian cell cycle proposed by Gérard and Gold beter (2011). The cell division occurs when the cyclinB/Cdk1 (cyclin-dependent kinase) complex is totally degraded and it reaches a minimum value. At this point, the cell is divided into two newborn daughter cells and each one will contain the half of the cyto plasmic content of the mother cell. The equations of our base model are valid only if the cell volume, where the reactions occur, is constant. Whether the cell volume is not constant, that is, the rate of change of its volume with respect to time is explicitly taken into account in the mathematical model, then the equations of the original model are no longer valid. Therefore, every equations were modified from the mass conservation prin ciple for considering a volume that changes with time. Through this approach, the cell volume affects all model variables. Two different dynamic simulation methods were ac complished: deterministic and stochastic. In the stochastic simulation, the volume affects every model’s parameters which have molar unit, whereas in the deterministic one, it is incorporated into the differential equations. In deterministic simulation, the biochemical species may be in concentration units, while in stochastic simulation such species must be converted to number of molecules which are directly proportional to the cell volume. In an effort to understand the influence of the new equation over the model an stability analysis was performed. This elucidates how the new parameter µ, cell volume growth factor, impacts the stability of the model’s limit cycle. In order to find the approximated solution of the deterministic model, the fourth order Runge Kutta method was implemen ted. As for the stochastic model, the Gillespie’s Direct Method was used. In conclusion, a more precise model, in comparison to the base model, was created for the cell cycle as it now takes into consideration the rate of change of the cell volume.

Ciclo celular

Simulação estocástica

Simulação determinista

Volume celular variável

Cell Cycle

Stochastic Simulation

Deterministic Simulation

Variable Cell Volume

Effects of xylazine, romifidine and detomidine on haematology, serum biochemistry and splenic size in horses

Kullmann, Anne

30 November 2011

Alpha 2 agonists are frequently used in equine medicine. This study focused primarily on α2 agonist-induced changes in PCV and TSP. A secondary aim of this study was to investigate the effects of α2 agonist on selected serum biochemical parameters and splenic size in order to identify potential causes for the changes seen in PCV and TSP. Four healthy adult mares were treated in a blinded, randomized, cross-over design with a single dose of xylazine (0.5 mg/kg), romifidine (0.04 mg/kg) or detomidine (0.01 mg/kg) intravenously, or detomidine (0.02 mg/kg) intramuscularly. A 1-week washout period was allowed between treatments. Haematology, TSP, COP, plasma osmolality, glucose, BUN, serum lactate, electrolytes, venous blood pH, ultrasonographic splenic size and degree of clinical sedation were evaluated at different time points post-injection and compared to baseline values. All treatments induced similar clinical sedation in the mares. A significant change over time in PCV and TSP following each treatment was identified, with overall median (range) maximal reductions compared to baseline of 20.9% (12.9 - 27.3%) and 5.8% (3.0 - 10.3%), respectively. Additionally, changes over time were significant for RBC count, BUN, COP and Ca2+, which decreased; and glucose, plasma osmolality, Na+ and splenic size, which increased, when compared to baseline. There was no significant main effect of treatment on PCV, TSP or any other parameters measured except for glucose. This study concluded that changes in PCV, TSP and other biochemical parameters induced by α2 agonists should be taken into consideration when assessing critically ill horses that received these drugs. There was evidence of splenic RBC sequestration as well as fluid shifts; therefore, the results suggest a multifactorial cause for the changes in PCV and TSP. / Dissertation (MSc)--University of Pretoria, 2011. / Companion Animal Clinical Studies / unrestricted

Colloid osmotic pressure

Plasma osmolality

Total serum protein

Packed cell volume

Splenic size

Alpha 2 adrenoceptor agonist

Horses

Xylazine

Detomidine

Romifidine

UCTD

Objemově regulované aniontové kanály u astrocytů - in vitro and in situ analýza / Volume-regulated anion channels in astrocytes- in vitro and in situ analysis

Harantová, Lenka

January 2012

Astrocytes need to preserve constant volume in the face of osmolarity perturbations to function properly. To regain their original volume after hyposmotically induced swelling, they extrude intracellular electrolytes and organic osmolytes, such as inorganic ions, excitative amino acids or polyols, accompanied by osmotically driven water. This process is termed regulatory volume decrease and is ensured by various ion channels and transporters. Recently, much attention has been focused on the ubiquitous volume-regulated anion channels activated by cell swelling. VRACs are moderately outwardly rectifying with intermediary conductance, permeable to inorganic anions and organic osmolytes and sensitive to broad-spectrum anion channels blockers. Using patch-clamp technique we aimed to characterize VRACs in cultured cortical astrocytes isolated from neonatal Wistar rats and to elucidate the effect of intracellular Na+ on VRAC activity. In addition, we also intended to characterize these channels in situ in brain slices of 10 - 12 days old rats, focusing mainly on hippocampal astrocytes. To induce astrocytic swelling, we exposed astrocytes to hypotonic solution (250 mOsm). In agreement with previous findings, we showed that cultured cortical astrocytes activate VRAC currents upon exposure to hypotonic stress, which...

Évaluation des effets de l'administration de fer intramusculaire sur l'anémie chez les oiseaux de proie

Dubé, Catherine

04 1900

L’administration de fer dextran à 10 mg/kg intramusculaire (IM) est un traitement empirique couramment recommandé en médecine aviaire lors d’hémorragie ou d’anémie. L’objectif principal de cette étude était d’évaluer les effets de ce traitement sur l’anémie chez les oiseaux de proie. Deux types d’individus ont été utilisés : des crécerelles d’Amérique (Falco sparverius) où une anémie par perte de sang externe aiguë a été créée (deux phlébotomies de 20-40 % du volume sanguin total à un intervalle de 6 h) et des oiseaux de proie sauvages de différentes espèces souffrant d’anémies diverses. L’ensemble des oiseaux a été subdivisé aléatoirement en groupe traitement (fer dextran 10 mg/kg IM) et contrôle (NaCl 0,9% IM). Un suivi dans le temps a été réalisé afin d’étudier leur récupération de l’anémie, la présence d’effets secondaires au traitement et l’impact d’une administration de fer sur ces réserves. Aucune différence significative n’a été observée entre les deux groupes en ce qui concerne les signes cliniques, l’hématocrite, le pourcentage des polychromatophiles/réticulocytes, la densité cellulaire et le fer de la moelle osseuse, la créatine kinase et le fer plasmatique. La majorité des crécerelles ont présenté une myosite au site d’injection du fer. Nos résultats suggèrent qu’une administration de 10 mg/kg de fer dextran IM n’a pas d’effet sur l’érythropoïèse des rapaces souffrant d’anémie par perte de sang externe aiguë, qu’elle provoque une légère inflammation au site d’injection et qu’elle n’influence pas les réserves de fer. Le comptage des réticulocytes en anneau et des polychromatophiles semble être deux méthodes équivalentes. / A 10 mg/kg intramuscular (IM) administration of iron dextran is a common empirical treatment recommended in avian medicine for hemorrhage and anemia. The purpose of this study was to evaluate the effects of this treatment on anemia in birds of prey. Two kinds of specimen were used: the American kestrel (Falco sparverius) where an acute external blood loss anemia was created (with two phlebotomies of 20-40 % of the total blood volume at 6 hours interval) and other various species of wild birds of prey suffering from different types of anemia. All subjects were randomized into a treatment (iron dextran 10 mg/kg IM) or a control (NaCl 0,9 % IM) group. Monitoring was carried out to evaluate the evolution of the anemia, presence of side effects and impact of an iron administration on their iron reserve. No significant differences were observed between the two treatment groups for clinical signs, packed cell volume, the percentage of reticulocytes/polychromatophilic erythrocytes, bone marrow cellularity and iron, plasmatic iron and creatine kinase. Most kestrels had a myositis at the iron injection site. Our results suggest that an IM injection of 10 mg/kg iron dextran has no effect on raptor erythropoiesis after an acute external blood loss anemia, that it has no effect on iron reserve, and that it can cause mild inflammation at the injection site. The polychromatophilic erythrocytes and the reticulocytes ring form count were two equivalent methods.

Anémie

Fer dextran

Oiseaux de proie

Crécerelle d'Amérique

Hématocrite

Réticulocytes

Polychromatophiles

Moelle osseuse

Fer plasmatique

Anemia

Iron dextran

Birds of prey

American kestrel

Packed cell volume (PCV)

Reticulocytes

Polychromatophilic erythrocytes

Bone marrow

Plasmatic iron

Évaluation des effets de l'administration de fer intramusculaire sur l'anémie chez les oiseaux de proie

Dubé, Catherine

04 1900

L’administration de fer dextran à 10 mg/kg intramusculaire (IM) est un traitement empirique couramment recommandé en médecine aviaire lors d’hémorragie ou d’anémie. L’objectif principal de cette étude était d’évaluer les effets de ce traitement sur l’anémie chez les oiseaux de proie. Deux types d’individus ont été utilisés : des crécerelles d’Amérique (Falco sparverius) où une anémie par perte de sang externe aiguë a été créée (deux phlébotomies de 20-40 % du volume sanguin total à un intervalle de 6 h) et des oiseaux de proie sauvages de différentes espèces souffrant d’anémies diverses. L’ensemble des oiseaux a été subdivisé aléatoirement en groupe traitement (fer dextran 10 mg/kg IM) et contrôle (NaCl 0,9% IM). Un suivi dans le temps a été réalisé afin d’étudier leur récupération de l’anémie, la présence d’effets secondaires au traitement et l’impact d’une administration de fer sur ces réserves. Aucune différence significative n’a été observée entre les deux groupes en ce qui concerne les signes cliniques, l’hématocrite, le pourcentage des polychromatophiles/réticulocytes, la densité cellulaire et le fer de la moelle osseuse, la créatine kinase et le fer plasmatique. La majorité des crécerelles ont présenté une myosite au site d’injection du fer. Nos résultats suggèrent qu’une administration de 10 mg/kg de fer dextran IM n’a pas d’effet sur l’érythropoïèse des rapaces souffrant d’anémie par perte de sang externe aiguë, qu’elle provoque une légère inflammation au site d’injection et qu’elle n’influence pas les réserves de fer. Le comptage des réticulocytes en anneau et des polychromatophiles semble être deux méthodes équivalentes. / A 10 mg/kg intramuscular (IM) administration of iron dextran is a common empirical treatment recommended in avian medicine for hemorrhage and anemia. The purpose of this study was to evaluate the effects of this treatment on anemia in birds of prey. Two kinds of specimen were used: the American kestrel (Falco sparverius) where an acute external blood loss anemia was created (with two phlebotomies of 20-40 % of the total blood volume at 6 hours interval) and other various species of wild birds of prey suffering from different types of anemia. All subjects were randomized into a treatment (iron dextran 10 mg/kg IM) or a control (NaCl 0,9 % IM) group. Monitoring was carried out to evaluate the evolution of the anemia, presence of side effects and impact of an iron administration on their iron reserve. No significant differences were observed between the two treatment groups for clinical signs, packed cell volume, the percentage of reticulocytes/polychromatophilic erythrocytes, bone marrow cellularity and iron, plasmatic iron and creatine kinase. Most kestrels had a myositis at the iron injection site. Our results suggest that an IM injection of 10 mg/kg iron dextran has no effect on raptor erythropoiesis after an acute external blood loss anemia, that it has no effect on iron reserve, and that it can cause mild inflammation at the injection site. The polychromatophilic erythrocytes and the reticulocytes ring form count were two equivalent methods.

Anémie

Fer dextran

Oiseaux de proie

Crécerelle d'Amérique

Hématocrite

Réticulocytes

Polychromatophiles

Moelle osseuse

Fer plasmatique

Anemia

Iron dextran

Birds of prey

American kestrel

Packed cell volume (PCV)

Reticulocytes

Polychromatophilic erythrocytes

Bone marrow

Plasmatic iron

Shrinkage, Swelling and Macromolecular Crowding in Cell Death

Rana, Priyanka Shailendra

28 July 2020

No description available.

Biology

Physiology

Cellular Biology

Biophysics

Molecular Biology

Biochemistry

Macromolecular crowding

Cell volume

Volume sensing

Apoptotic shrinkage

Necrotic swelling

Ion probes

Ionophores

Intracellular potassium measurement

Quantitative phase imaging

Functions of the apical Na⁺/ K⁺/ 2Cl^- Cotransporter 1 in choroid plexus epithelial cells.

Gregoriades, Jeannine Marie Crum

01 September 2017

No description available.

Biomedical Research

Biophysics

Neurosciences

Physiology

choroid plexus

epithelial cells

cell volume measurements

NKCC1

NKCC1 KO mice

intracellular sodium

intracellular chloride

Calcein

MQAE

Asante natrium green

cerebrospinal fluid

extracellular potassium regulation

The Mechanics of Mitotic Cell Rounding

Stewart, Martin

11 July 2012

During mitosis, adherent animal cells undergo a drastic shape change, from essentially flat to round, in a process known as mitotic cell rounding (MCR). The aim of this thesis was to critically examine the physical and biological basis of MCR. The experimental part of this thesis employed a combined optical microscope-atomic force microscope (AFM) setup in conjunction with flat tipless cantilevers to analyze cell mechanics, shape and volume. To this end, two AFM assays were developed: the constant force assay (CFA), which applies constant force to cells and measures the resultant height, and the constant height assay (CHA), which confines cell height and measures the resultant force. These assays were deployed to analyze the shape and mechanical properties of single cells trans-mitosis. The CFA results showed that cells progressing through mitosis could increase their height against forces as high as 50 nN, and that higher forces can delay mitosis in HeLa cells. The CHA results showed that mitotic cells confined to ~50% of their normal height can generate forces around 50-100 nN without disturbing mitotic progression. Such forces represent intracellular pressures of at least 200 Pascals and cell surface tensions of around 10 nN/µm. Using the CHA to compare mitotic cell rounding with induced cell rounding, it was observed that the intracellular pressure of mitotic cells is at least 3-fold higher than rounded interphase cells. To investigate the molecular basis of the mechanical changes inherent in mitotic cell rounding, inhibitors and toxins were used to pharmacologically dissect the role of candidate cellular processes. These results implicated the actomyosin cortex and osmolyte transporters, the most prominent of which is the Na+/H+ exchanger, in the maintenance of mechanical properties and intracellular hydrostatic pressure. Observations on blebbing cells under the cantilever supported the idea that the actomyosin cortex is required to sustain hydrostatic pressure and direct this pressure into cell shape changes. To gain further insight into the relationship between actomyosin activity and intracellular pressure, dynamic perturbation experiments were conducted. To this end, the CHA was used to evaluate the pressure and volume of mitotic cells before, during and after dynamic perturbations that included tonic shocks, influx of specific inhibitors, and exposure to pore-forming toxins. When osmotic pressure gradients were depleted, pressure and volume decreased. When the actomyosin cytoskeleton was abolished, cell volume increased while rounding pressure decreased. Conversely, stimulation of actomyosin cortex contraction triggered an increase in rounding pressure and a decrease in volume. Taken together, the dynamic perturbation results demonstrated that the actomyosin cortex contracts against an opposing intracellular pressure and that this relationship sets the surface tension, pressure and volume of the cell. The discussion section of this thesis provides a comprehensive overview of the physical basis of MCR by amalgamating the experimental results of this thesis with the literature. Additionally, the biochemal signaling pathways and proteins that drive MCR are collated and discussed. An exhaustive and unprecedented synthesis of the literature on cell rounding (approx. 750 papers as pubmed search hits on “cell rounding”, April 2012) reveals that the spread-to-round transition can be thought of in terms of a surface tension versus adhesion paradigm, and that cell rounding can be physically classified into four main modes, of which one is an MCR-like category characterized by increased actomyosin cortex tension and diminution of focal adhesions. The biochemical pathways and signaling patterns that correspond with these four rounding modes are catalogued and expounded upon in the context of the relevant physiology. This analysis reveals cell rounding as a pertinent topic that can be leveraged to yield insight into core principles of cell biophysics and tissue organization. It furthermore highlights MCR as a model problem to understand the adhesion versus cell surface tension paradigm in cells and its fundamentality to cell shape, mechanics and physiology.

mitotische Zellabrundung

Zellabrundung

Mitose

Rasterkraftmikroskopie

AFM

Zell-Biophysik

Zellform

Zellphysiologie

Zell-Mechanik

Zellvolumen

intrazellulärer Druck

Actomyosin

Runden Kraft

Zelle Oberflächenspannung

Cortex Spannung

Zelladhäsion

mitotic cell rounding

cell rounding

mitosis

AFM

cell biophysics

cell shape

cell physiology

cell mechanics

cell volume

intracellular pressure

actomyosin

rounding force

cell surface tension

cortex tension

cell adhesion

ddc:570

rvk:WE 2100