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Cell growth

February 16, 2024

Cell growth refers to an increase in the total mass of a cell, including both cytoplasmic, nuclear and organelle volume.[1] Cell growth occurs when the overall rate of cellular biosynthesis (production of biomolecules or anabolism) is greater than the overall rate of cellular degradation (the destruction of biomolecules via the proteasome, lysosome or autophagy, or catabolism).[2][3][4]

Cell division, growth & proliferation

Cell growth is not to be confused with cell division or the cell cycle, which are distinct processes that can occur alongside cell growth during the process of cell proliferation, where a cell, known as the mother cell, grows and divides to produce two daughter cells.[1] Importantly, cell growth and cell division can also occur independently of one another. During early embryonic development (cleavage of the zygote to form a morula and blastoderm), cell divisions occur repeatedly without cell growth. Conversely, some cells can grow without cell division or without any progression of the cell cycle, such as growth of neurons during axonal pathfinding in nervous system development.

Cell division without cell growth during embryonic cleavage

In multicellular organisms, tissue growth rarely occurs solely through cell growth without cell division, but most often occurs through cell proliferation.[1] This is because a single cell with only one copy of the genome in the cell nucleus can perform biosynthesis and thus undergo cell growth at only half the rate of two cells. Hence, two cells grow (accumulate mass) at twice the rate of a single cell, and four cells grow at 4-times the rate of a single cell. This principle leads to an exponential increase of tissue growth rate (mass accumulation) during cell proliferation, owing to the exponential increase in cell number.

Cell size depends on both cell growth and cell division, with a disproportionate increase in the rate of cell growth leading to production of larger cells and a disproportionate increase in the rate of cell division leading to production of many smaller cells. Cell proliferation typically involves balanced cell growth and cell division rates that maintain a roughly constant cell size in the exponentially proliferating population of cells.

Some special cells can grow to very large sizes via an unusual endoreplication cell cycle in which the genome is replicated during S-phase but there is no subsequent mitosis (M-phase) or cell division (cytokinesis). These large endoreplicating cells have many copies of the genome, so are highly polyploid.

Oocytes can be unusually large cells in species for which embryonic development takes place away from the mother's body within an egg that is laid externally. The large size of some eggs can be achieved either by pumping in cytosolic components from adjacent cells through cytoplasmic bridges named ring canals (Drosophila) or by internalisation of nutrient storage granules (yolk granules) by endocytosis (frogs).

Mechanisms of cell growth control edit

Cells can grow by increasing the overall rate of cellular biosynthesis such that production of biomolecules exceeds the overall rate of cellular degradation of biomolecules via the proteasome, lysosome or autophagy.

Biosynthesis of biomolecules is initiated by expression of genes which encode RNAs and/or proteins, including enzymes that catalyse synthesis of lipids and carbohydrates.

Individual genes are generally expressed via transcription into messenger RNA (mRNA) and translation into proteins, and the expression of each gene occurs to various different levels in a cell-type specific fashion (in response to gene regulatory networks).

To drive cell growth, the global rate of gene expression can be increased by enhancing the overall rate of transcription by RNA polymerase II (for active genes) or the overall rate of mRNA translation into protein by increasing the abundance of ribosomes and tRNA, whose biogenesis depends on RNA polymerase I and RNA polymerase III. The Myc transcription factor is an example of a regulatory protein that can induce the overall activity of RNA polymerase I, RNA polymerase II and RNA polymerase III to drive global transcription and translation and thereby cell growth.

In addition, the activity of individual ribosomes can be increased to boost the global efficiency of mRNA translation via regulation of translation initiation factors, including the 'translational elongation initiation factor 4E' (eIF4E) complex, which binds to and caps the 5' end of mRNAs. The protein TOR, part of the TORC1 complex, is an important upstream regulator of translation initiation as well as ribosome biogenesis.[5] TOR is a serine/threonine kinase that can directly phosphorylate and inactivate a general inhibitor of eIF4E, named 4E-binding protein (4E-BP), to promote translation efficiency. TOR also directly phosphorylates and activates the ribosomal protein S6-kinase (S6K), which promotes ribosome biogenesis.

To inhibit cell growth, the global rate of gene expression can be decreased or the global rate of biomolecular degradation can be increased by increasing the rate of autophagy. TOR normally directly inhibits the function of the autophagy inducing kinase Atg1/ULK1. Thus, reducing TOR activity both reduces the global rate of translation and increases the extent of autophagy to reduce cell growth.

Cell growth regulation in animals edit

Many of the signal molecules that control of cellular growth are called growth factors, many of which induce signal transduction via the PI3K/AKT/mTOR pathway, which includes upstream lipid kinase PI3K and the downstream serine/threonine protein kinase Akt, which is able to activate another protein kinase TOR, which promotes translation and inhibits autophagy to drive cell growth.

Nutrient availability influences production of growth factors of the Insulin/IGF-1 family, which circulate as hormones in animals to activate the PI3K/AKT/mTOR pathway in cells to promote TOR activity so that when animals are well fed they will grow rapidly and when they are not able to receive sufficient nutrients they will reduce their growth rate. Recently it has been also demonstrated that cellular bicarbonate metabolism, which is responsible for cell growth, can be regulated by mTORC1 signaling.[6]

In addition, the availability of amino acids to individual cells also directly promotes TOR activity, although this mode of regulation is more important in single-celled organisms than in multicellular organisms such as animals that always maintain an abundance of amino acids in circulation.

One disputed theory proposes that many different mammalian cells undergo size-dependent transitions during the cell cycle. These transitions are controlled by the cyclin-dependent kinase Cdk1.[7] Though the proteins that control Cdk1 are well understood, their connection to mechanisms monitoring cell size remains elusive.

A postulated model for mammalian size control situates mass as the driving force of the cell cycle. A cell is unable to grow to an abnormally large size because at a certain cell size or cell mass, the S phase is initiated. The S phase starts the sequence of events leading to mitosis and cytokinesis. A cell is unable to get too small because the later cell cycle events, such as S, G2, and M, are delayed until mass increases sufficiently to begin S phase.[8]

Cell populations edit

Cell populations go through a particular type of exponential growth called doubling or cell proliferation. Thus, each generation of cells should be twice as numerous as the previous generation. However, the number of generations only gives a maximum figure as not all cells survive in each generation. Cells can reproduce in the stage of Mitosis, where they double and split into two genetically equal cells.

Cell size edit

Cell size is highly variable among organisms, with some algae such as Caulerpa taxifolia being a single cell several meters in length.[9] Plant cells are much larger than animal cells, and protists such as Paramecium can be 330 μm long, while a typical human cell might be 10 μm. How these cells "decide" how big they should be before dividing is an open question. Chemical gradients are known to be partly responsible, and it is hypothesized that mechanical stress detection by cytoskeletal structures is involved. Work on the topic generally requires an organism whose cell cycle is well-characterized.

Yeast cell size regulation edit

The relationship between cell size and cell division has been extensively studied in yeast. For some cells, there is a mechanism by which cell division is not initiated until a cell has reached a certain size. If the nutrient supply is restricted (after time t = 2 in the diagram, below), and the rate of increase in cell size is slowed, the time period between cell divisions is increased.[10] Yeast cell-size mutants were isolated that begin cell division before reaching a normal/regular size (wee mutants).[11]

 
Figure 1:Cell cycle and growth

Wee1 protein is a tyrosine kinase that normally phosphorylates the Cdc2 cell cycle regulatory protein (the homolog of CDK1 in humans), a cyclin-dependent kinase, on a tyrosine residue. Cdc2 drives entry into mitosis by phosphorylating a wide range of targets. This covalent modification of the molecular structure of Cdc2 inhibits the enzymatic activity of Cdc2 and prevents cell division. Wee1 acts to keep Cdc2 inactive during early G2 when cells are still small. When cells have reached sufficient size during G2, the phosphatase Cdc25 removes the inhibitory phosphorylation, and thus activates Cdc2 to allow mitotic entry. A balance of Wee1 and Cdc25 activity with changes in cell size is coordinated by the mitotic entry control system. It has been shown in Wee1 mutants, cells with weakened Wee1 activity, that Cdc2 becomes active when the cell is smaller. Thus, mitosis occurs before the yeast reach their normal size. This suggests that cell division may be regulated in part by dilution of Wee1 protein in cells as they grow larger.

Linking Cdr2 to Wee1 edit

The protein kinase Cdr2 (which negatively regulates Wee1) and the Cdr2-related kinase Cdr1 (which directly phosphorylates and inhibits Wee1 in vitro)[12] are localized to a band of cortical nodes in the middle of interphase cells. After entry into mitosis, cytokinesis factors such as myosin II are recruited to similar nodes; these nodes eventually condense to form the cytokinetic ring.[13] A previously uncharacterized protein, Blt1, was found to colocalize with Cdr2 in the medial interphase nodes. Blt1 knockout cells had increased length at division, which is consistent with a delay in mitotic entry. This finding connects a physical location, a band of cortical nodes, with factors that have been shown to directly regulate mitotic entry, namely Cdr1, Cdr2, and Blt1.

Further experimentation with GFP-tagged proteins and mutant proteins indicates that the medial cortical nodes are formed by the ordered, Cdr2-dependent assembly of multiple interacting proteins during interphase. Cdr2 is at the top of this hierarchy and works upstream of Cdr1 and Blt1.[14] Mitosis is promoted by the negative regulation of Wee1 by Cdr2. It has also been shown that Cdr2 recruits Wee1 to the medial cortical node. The mechanism of this recruitment has yet to be discovered. A Cdr2 kinase mutant, which is able to localize properly despite a loss of function in phosphorylation, disrupts the recruitment of Wee1 to the medial cortex and delays entry into mitosis. Thus, Wee1 localizes with its inhibitory network, which demonstrates that mitosis is controlled through Cdr2-dependent negative regulation of Wee1 at the medial cortical nodes.[14]

Cell polarity factors edit

Cell polarity factors positioned at the cell tips provide spatial cues to limit Cdr2 distribution to the cell middle. In fission yeast Schizosaccharomyces pombe (S. Pombe), cells divide at a defined, reproducible size during mitosis because of the regulated activity of Cdk1.[15] The cell polarity protein kinase Pom1, a member of the dual-specificity tyrosine-phosphorylation regulated kinase (DYRK) family of kinases, localizes to cell ends. In Pom1 knockout cells, Cdr2 was no longer restricted to the cell middle, but was seen diffusely through half of the cell. From this data it becomes apparent that Pom1 provides inhibitory signals that confine Cdr2 to the middle of the cell. It has been further shown that Pom1-dependent signals lead to the phosphorylation of Cdr2. Pom1 knockout cells were also shown to divide at a smaller size than wild-type, which indicates a premature entry into mitosis.[14]

Pom1 forms polar gradients that peak at cell ends, which shows a direct link between size control factors and a specific physical location in the cell.[16] As a cell grows in size, a gradient in Pom1 grows. When cells are small, Pom1 is spread diffusely throughout the cell body. As the cell increases in size, Pom1 concentration decreases in the middle and becomes concentrated at cell ends. Small cells in early G2 which contain sufficient levels of Pom1 in the entirety of the cell have inactive Cdr2 and cannot enter mitosis. It is not until the cells grow into late G2, when Pom1 is confined to the cell ends that Cdr2 in the medial cortical nodes is activated and able to start the inhibition of Wee1. This finding shows how cell size plays a direct role in regulating the start of mitosis. In this model, Pom1 acts as a molecular link between cell growth and mitotic entry through a Cdr2-Cdr1-Wee1-Cdk1 pathway.[14] The Pom1 polar gradient successfully relays information about cell size and geometry to the Cdk1 regulatory system. Through this gradient, the cell ensures it has reached a defined, sufficient size to enter mitosis.

Other experimental systems for the study of cell size regulation edit

One common means to produce very large cells is by cell fusion to form syncytia. For example, very long (several inches) skeletal muscle cells are formed by fusion of thousands of myocytes. Genetic studies of the fruit fly Drosophila have revealed several genes that are required for the formation of multinucleated muscle cells by fusion of myoblasts.[17] Some of the key proteins are important for cell adhesion between myocytes and some are involved in adhesion-dependent cell-to-cell signal transduction that allows for a cascade of cell fusion events.

Increases in the size of plant cells are complicated by the fact that almost all plant cells are inside of a solid cell wall. Under the influence of certain plant hormones the cell wall can be remodeled, allowing for increases in cell size that are important for the growth of some plant tissues.

Most unicellular organisms are microscopic in size, but there are some giant bacteria and protozoa that are visible to the naked eye. (See Table of cell sizes—Dense populations of a giant sulfur bacterium in Namibian shelf sediments[18]—.)

In the rod-shaped bacteria E. coli, Caulobacter crescentus and B. subtilis cell size is controlled by a simple mechanisms in which cell division occurs after a constant volume has been added since the previous division.[19][20] By always growing by the same amount, cells born smaller or larger than average naturally converge to an average size equivalent to the amount added during each generation.

Cell division edit

Cell reproduction is asexual. For most of the constituents of the cell, growth is a steady, continuous process, interrupted only briefly at M phase when the nucleus and then the cell divide in two.

The process of cell division, called cell cycle, has four major parts called phases. The first part, called G1 phase is marked by synthesis of various enzymes that are required for DNA replication. The second part of the cell cycle is the S phase, where DNA replication produces two identical sets of chromosomes. The third part is the G2 phase in which a significant protein synthesis occurs, mainly involving the production of microtubules that are required during the process of division, called mitosis. The fourth phase, M phase, consists of nuclear division (karyokinesis) and cytoplasmic division (cytokinesis), accompanied by the formation of a new cell membrane. This is the physical division of mother and daughter cells. The M phase has been broken down into several distinct phases, sequentially known as prophase, prometaphase, metaphase, anaphase and telophase leading to cytokinesis.

Cell division is more complex in eukaryotes than in other organisms. Prokaryotic cells such as bacterial cells reproduce by binary fission, a process that includes DNA replication, chromosome segregation, and cytokinesis. Eukaryotic cell division either involves mitosis or a more complex process called meiosis. Mitosis and meiosis are sometimes called the two nuclear division processes. Binary fission is similar to eukaryote cell reproduction that involves mitosis. Both lead to the production of two daughter cells with the same number of chromosomes as the parental cell. Meiosis is used for a special cell reproduction process of diploid organisms. It produces four special daughter cells (gametes) which have half the normal cellular amount of DNA. A male and a female gamete can then combine to produce a zygote, a cell which again has the normal amount of chromosomes.

The rest of this article is a comparison of the main features of the three types of cell reproduction that either involve binary fission, mitosis, or meiosis. The diagram below depicts the similarities and differences of these three types of cell reproduction.

 
Cell growth

Comparison of the three types of cell division edit

The DNA content of a cell is duplicated at the start of the cell reproduction process. Prior to DNA replication, the DNA content of a cell can be represented as the amount Z (the cell has Z chromosomes). After the DNA replication process, the amount of DNA in the cell is 2Z (multiplication: 2 x Z = 2Z). During Binary fission and mitosis the duplicated DNA content of the reproducing parental cell is separated into two equal halves that are destined to end up in the two daughter cells. The final part of the cell reproduction process is cell division, when daughter cells physically split apart from a parental cell. During meiosis, there are two cell division steps that together produce the four daughter cells.

After the completion of binary fission or cell reproduction involving mitosis, each daughter cell has the same amount of DNA (Z) as what the parental cell had before it replicated its DNA. These two types of cell reproduction produced two daughter cells that have the same number of chromosomes as the parental cell. Chromosomes duplicate prior to cell division when forming new skin cells for reproduction. After meiotic cell reproduction the four daughter cells have half the number of chromosomes that the parental cell originally had. This is the haploid amount of DNA, often symbolized as N. Meiosis is used by diploid organisms to produce haploid gametes. In a diploid organism such as the human organism, most cells of the body have the diploid amount of DNA, 2N. Using this notation for counting chromosomes we say that human somatic cells have 46 chromosomes (2N = 46) while human sperm and eggs have 23 chromosomes (N = 23). Humans have 23 distinct types of chromosomes, the 22 autosomes and the special category of sex chromosomes. There are two distinct sex chromosomes, the X chromosome and the Y chromosome. A diploid human cell has 23 chromosomes from that person's father and 23 from the mother. That is, your body has two copies of human chromosome number 2, one from each of your parents.

 
Chromosomes

Immediately after DNA replication a human cell will have 46 "double chromosomes". In each double chromosome there are two copies of that chromosome's DNA molecule. During mitosis the double chromosomes are split to produce 92 "single chromosomes", half of which go into each daughter cell. During meiosis, there are two chromosome separation steps which assure that each of the four daughter cells gets one copy of each of the 23 types of chromosome.

Sexual reproduction edit

Main article: Evolution of sex
Further information: Origin and function of meiosis and Homologous recombination

Though cell reproduction that uses mitosis can reproduce eukaryotic cells, eukaryotes bother with the more complicated process of meiosis because sexual reproduction such as meiosis confers a selective advantage. Notice that when meiosis starts, the two copies of sister chromatids number 2 are adjacent to each other. During this time, there can be genetic recombination events. Information from the chromosome 2 DNA gained from one parent (red) will transfer over to the chromosome 2 DNA molecule that was received from the other parent (green). Notice that in mitosis the two copies of chromosome number 2 do not interact. Recombination of genetic information between homologous chromosomes during meiosis is a process for repairing DNA damages. This process can also produce new combinations of genes, some of which may be adaptively beneficial and influence the course of evolution. However, in organisms with more than one set of chromosomes at the main life cycle stage, sex may also provide an advantage because, under random mating, it produces homozygotes and heterozygotes according to the Hardy–Weinberg ratio.

Disorders edit

A series of growth disorders can occur at the cellular level and these consequently underpin much of the subsequent course in cancer, in which a group of cells display uncontrolled growth and division beyond the normal limits, invasion (intrusion on and destruction of adjacent tissues), and sometimes metastasis (spread to other locations in the body via lymph or blood). Several key determinants of cell growth, like ploidy and the regulation of cellular metabolism, are commonly disrupted in tumors.[21] Therefore, heterogenous cell growth and pleomorphism is one of the earliest hallmarks of cancer progression.[22][23] Despite the prevalence of pleomorphism in human pathology, its role in disease progression is unclear. In epithelial tissues, misregulation of cellular size can induce packing defects and disperse aberrant cells.[24] But the consequence of atypical cell growth in other animal tissues is unknown.

Measurement methods edit

The cell growth can be detected by a variety of methods. The cell size growth can be visualized by microscopy, using suitable stains. But the increase of cells number is usually more significant. It can be measured by manual counting of cells under microscopy observation, using the dye exclusion method (i.e. trypan blue) to count only viable cells. Less fastidious, scalable, methods include the use of cytometers, while flow cytometry allows combining cell counts ('events') with other specific parameters: fluorescent probes for membranes, cytoplasm or nuclei allow distinguishing dead/viable cells, cell types, cell differentiation, expression of a biomarker such as Ki67.

Beside the increasing number of cells, one can be assessed regarding the metabolic activity growth, that is, the CFDA and calcein-AM measure (fluorimetrically) not only the membrane functionality (dye retention), but also the functionality of cytoplasmic enzymes (esterases). The MTT assays (colorimetric) and the resazurin assay (fluorimetric) dose the mitochondrial redox potential.

All these assays may correlate well, or not, depending on cell growth conditions and desired aspects (activity, proliferation). The task is even more complicated with populations of different cells, furthermore when combining cell growth interferences or toxicity.

See also edit

References edit

  1. ^ a b c Conlon, Ian; Raff, Martin (1999). "Size Control in Animal Development". Cell. 96 (2): 235–244. doi:10.1016/S0092-8674(00)80563-2. ISSN 0092-8674. PMID 9988218. S2CID 15738174.
  2. ^ Grewal, Savraj S; Edgar, Bruce A (2003). "Controlling cell division in yeast and animals: does size matter?". Journal of Biology. 2 (1): 5. doi:10.1186/1475-4924-2-5. ISSN 1475-4924. PMC 156596. PMID 12733996.
  3. ^ Neufeld, Thomas P; de la Cruz, Aida Flor A; Johnston, Laura A; Edgar, Bruce A (1998). "Coordination of Growth and Cell Division in the Drosophila Wing". Cell. 93 (7): 1183–1193. doi:10.1016/S0092-8674(00)81462-2. ISSN 0092-8674. PMID 9657151. S2CID 14608744.
  4. ^ Thompson, Barry J. (2010). "Developmental control of cell growth and division in Drosophila". Current Opinion in Cell Biology. 22 (6): 788–794. doi:10.1016/j.ceb.2010.08.018. PMID 20833011.
  5. ^ Hafen, E. (2004). "Interplay Between Growth Factor and Nutrient Signaling: Lessons from Drosophila TOR". TOR. Current Topics in Microbiology and Immunology. Vol. 279. pp. 153–167. doi:10.1007/978-3-642-18930-2_10. ISBN 978-3-642-62360-8. ISSN 0070-217X. PMID 14560957.
  6. ^ Ali E, Liponska A, O'Hara B, Amici D, Torno M, Gao P, Asara J, Yap M-N F, Mendillo M, Ben-Sahra I (June 2022). "The mTORC1-SLC4A7 axis stimulates bicarbonate import to enhance de novo nucleotide synthesis". Molecular Cell. 82 (1): 3284–3298.e7. doi:10.1016/j.molcel.2022.06.008. PMC 9444906. PMID 35772404.
  7. ^ Mitchison JM (2003). "Growth during the cell cycle". Int. Rev. Cytol. International Review of Cytology. 226: 165–258. doi:10.1016/S0074-7696(03)01004-0. ISBN 978-0-12-364630-9. PMID 12921238.
  8. ^ Cooper, Stephen (2004). "Control and maintenance of mammalian cell size". BMC Cell Biology. 5 (1): 35. doi:10.1186/1471-2121-5-35. PMC 524481. PMID 15456512.
  9. ^ Peplow, Mark (23 March 2005). "Algae create glue to repair cell damage". Nature.com. Retrieved 4 July 2016.
  10. ^ Slavov N.; Botstein D. (June 2011). "Coupling among Growth Rate Response, Metabolic Cycle and Cell Division Cycle in Yeast". Molecular Biology of the Cell. 22 (12): 1997–2009. doi:10.1091/mbc.E11-02-0132. PMC 3113766. PMID 21525243.
  11. ^ Wee1 mutants of S. pombe have small cell size and the homologous proteins in humans also regulate cell entry into mitosis; in Lodish HF, Berk A, Zipursky LS, Matsudaira P, et al., eds. (2000). Molecular cell biology (4th ed.). New York: W.H. Freeman. ISBN 978-0-7167-3136-8.
  12. ^ Wu L, Russell P (June 1993). "Nim1 kinase promotes mitosis by inactivating Wee1 tyrosine kinase". Nature. 363 (6431): 738–41. Bibcode:1993Natur.363..738W. doi:10.1038/363738a0. PMID 8515818. S2CID 4320080.
  13. ^ Wu JQ, Kuhn JR, Kovar DR, Pollard TD (November 2003). "Spatial and temporal pathway for assembly and constriction of the contractile ring in fission yeast cytokinesis". Dev. Cell. 5 (5): 723–34. doi:10.1016/S1534-5807(03)00324-1. PMID 14602073.
  14. ^ a b c d Moseley JB, Mayeux A, Paoletti A, Nurse P (June 2009). "A spatial gradient coordinates cell size and mitotic entry in fission yeast". Nature. 459 (7248): 857–60. Bibcode:2009Natur.459..857M. doi:10.1038/nature08074. PMID 19474789. S2CID 4330336.
  15. ^ Rupes I (September 2002). "Checking cell size in yeast". Trends Genet. 18 (9): 479–85. doi:10.1016/S0168-9525(02)02745-2. PMID 12175809.
  16. ^ Padte NN, Martin SG, Howard M, Chang F (December 2006). "The cell-end factor pom1p inhibits mid1p in specification of the cell division plane in fission yeast". Curr. Biol. 16 (24): 2480–7. doi:10.1016/j.cub.2006.11.024. PMID 17140794.
  17. ^ Menon SD, Osman Z, Chenchill K, Chia W (June 2005). "A positive feedback loop between Dumbfounded and Rolling pebbles leads to myotube enlargement in Drosophila". J. Cell Biol. 169 (6): 909–20. doi:10.1083/jcb.200501126. PMC 2171639. PMID 15955848.
  18. ^ Schulz HN, Brinkhoff T, Ferdelman TG, Mariné MH, Teske A, Jorgensen BB (April 1999). "Dense populations of a giant sulfur bacterium in Namibian shelf sediments". Science. 284 (5413): 493–5. Bibcode:1999Sci...284..493S. doi:10.1126/science.284.5413.493. PMID 10205058. S2CID 32571118.
  19. ^ Taheri-Araghi, S; Bradde, S; Sauls, J. T.; Hill, N. S.; Levin, P. A.; Paulsson, J; Vergassola, M; Jun, S (February 2015). "Cell-size control and homeostasis in bacteria". Current Biology. 25 (3): 385–391. doi:10.1016/j.cub.2014.12.009. PMC 4323405. PMID 25544609.
  20. ^ Campos, M; Surovtsev, I. V.; Kato, S; Paintdakhi, A; Beltran, B; Ebmeier, S. E.; Jacobs-Wagner, C (December 2014). "A constant size extension drives bacterial cell size homeostasis". Cell. 159 (6): 1433–1446. doi:10.1016/j.cell.2014.11.022. PMC 4258233. PMID 25480302.
  21. ^ Schmoller, Kurt M.; Skotheim, Jan M. (December 2015). "The Biosynthetic Basis of Cell Size Control". Trends Cell Biol. 25 (12): 793–802. doi:10.1016/j.tcb.2015.10.006. PMC 6773270. PMID 26573465.
  22. ^ Travis, W.D.; Brambilla, B.; Burke, A.P; Marx, A.; Nicholson, A.G. (2015). WHO Classification of Tumours of the Lung, Pleura, Thymus and Heart. Lyon: International Agency for Research on Cancer. ISBN 978-92-832-2436-5.
  23. ^ El-Naggar, A.K.; Chan, J.C.K.; Grandis, J.R.; Takata, T.; Slootweg, P.J. (2017-01-23). . Lyon: International Agency for Research on Cancer (also known as Adman). ISBN 978-92-832-2438-9. Archived from the original on 2019-10-31. Retrieved 2019-10-31.
  24. ^ Ramanathan, Subramanian P.; Krajnc, Matej; Gibson, Matthew C. (October 2019). "Cell-Size Pleomorphism Drives Aberrant Clone Dispersal in Proliferating Epithelia". Developmental Cell. 51 (1): 49–61.e4. doi:10.1016/j.devcel.2019.08.005. PMC 6903429. PMID 31495693.

Books edit

  • Morgan, David O. (2007). The cell cycle: principles of control. London: Sunderland, Mass. ISBN 978-0-9539181-2-6.

External links edit

  • A comparison of generational and exponential models of cell population growth
  • Local Growth in an Array of Disks Wolfram Demonstrations Project

February 16, 2024
cell, growth, refers, increase, total, mass, cell, including, both, cytoplasmic, nuclear, organelle, volume, occurs, when, overall, rate, cellular, biosynthesis, production, biomolecules, anabolism, greater, than, overall, rate, cellular, degradation, destruct. Cell growth refers to an increase in the total mass of a cell including both cytoplasmic nuclear and organelle volume 1 Cell growth occurs when the overall rate of cellular biosynthesis production of biomolecules or anabolism is greater than the overall rate of cellular degradation the destruction of biomolecules via the proteasome lysosome or autophagy or catabolism 2 3 4 Cell division growth amp proliferationCell growth is not to be confused with cell division or the cell cycle which are distinct processes that can occur alongside cell growth during the process of cell proliferation where a cell known as the mother cell grows and divides to produce two daughter cells 1 Importantly cell growth and cell division can also occur independently of one another During early embryonic development cleavage of the zygote to form a morula and blastoderm cell divisions occur repeatedly without cell growth Conversely some cells can grow without cell division or without any progression of the cell cycle such as growth of neurons during axonal pathfinding in nervous system development Cell division without cell growth during embryonic cleavageIn multicellular organisms tissue growth rarely occurs solely through cell growth without cell division but most often occurs through cell proliferation 1 This is because a single cell with only one copy of the genome in the cell nucleus can perform biosynthesis and thus undergo cell growth at only half the rate of two cells Hence two cells grow accumulate mass at twice the rate of a single cell and four cells grow at 4 times the rate of a single cell This principle leads to an exponential increase of tissue growth rate mass accumulation during cell proliferation owing to the exponential increase in cell number Cell size depends on both cell growth and cell division with a disproportionate increase in the rate of cell growth leading to production of larger cells and a disproportionate increase in the rate of cell division leading to production of many smaller cells Cell proliferation typically involves balanced cell growth and cell division rates that maintain a roughly constant cell size in the exponentially proliferating population of cells Some special cells can grow to very large sizes via an unusual endoreplication cell cycle in which the genome is replicated during S phase but there is no subsequent mitosis M phase or cell division cytokinesis These large endoreplicating cells have many copies of the genome so are highly polyploid Oocytes can be unusually large cells in species for which embryonic development takes place away from the mother s body within an egg that is laid externally The large size of some eggs can be achieved either by pumping in cytosolic components from adjacent cells through cytoplasmic bridges named ring canals Drosophila or by internalisation of nutrient storage granules yolk granules by endocytosis frogs Contents 1 Mechanisms of cell growth control 2 Cell growth regulation in animals 3 Cell populations 4 Cell size 4 1 Yeast cell size regulation 4 1 1 Linking Cdr2 to Wee1 4 1 2 Cell polarity factors 4 2 Other experimental systems for the study of cell size regulation 5 Cell division 5 1 Comparison of the three types of cell division 5 2 Sexual reproduction 6 Disorders 7 Measurement methods 8 See also 9 References 10 Books 11 External linksMechanisms of cell growth control editCells can grow by increasing the overall rate of cellular biosynthesis such that production of biomolecules exceeds the overall rate of cellular degradation of biomolecules via the proteasome lysosome or autophagy Biosynthesis of biomolecules is initiated by expression of genes which encode RNAs and or proteins including enzymes that catalyse synthesis of lipids and carbohydrates Individual genes are generally expressed via transcription into messenger RNA mRNA and translation into proteins and the expression of each gene occurs to various different levels in a cell type specific fashion in response to gene regulatory networks To drive cell growth the global rate of gene expression can be increased by enhancing the overall rate of transcription by RNA polymerase II for active genes or the overall rate of mRNA translation into protein by increasing the abundance of ribosomes and tRNA whose biogenesis depends on RNA polymerase I and RNA polymerase III The Myc transcription factor is an example of a regulatory protein that can induce the overall activity of RNA polymerase I RNA polymerase II and RNA polymerase III to drive global transcription and translation and thereby cell growth In addition the activity of individual ribosomes can be increased to boost the global efficiency of mRNA translation via regulation of translation initiation factors including the translational elongation initiation factor 4E eIF4E complex which binds to and caps the 5 end of mRNAs The protein TOR part of the TORC1 complex is an important upstream regulator of translation initiation as well as ribosome biogenesis 5 TOR is a serine threonine kinase that can directly phosphorylate and inactivate a general inhibitor of eIF4E named 4E binding protein 4E BP to promote translation efficiency TOR also directly phosphorylates and activates the ribosomal protein S6 kinase S6K which promotes ribosome biogenesis To inhibit cell growth the global rate of gene expression can be decreased or the global rate of biomolecular degradation can be increased by increasing the rate of autophagy TOR normally directly inhibits the function of the autophagy inducing kinase Atg1 ULK1 Thus reducing TOR activity both reduces the global rate of translation and increases the extent of autophagy to reduce cell growth Cell growth regulation in animals editMany of the signal molecules that control of cellular growth are called growth factors many of which induce signal transduction via the PI3K AKT mTOR pathway which includes upstream lipid kinase PI3K and the downstream serine threonine protein kinase Akt which is able to activate another protein kinase TOR which promotes translation and inhibits autophagy to drive cell growth Nutrient availability influences production of growth factors of the Insulin IGF 1 family which circulate as hormones in animals to activate the PI3K AKT mTOR pathway in cells to promote TOR activity so that when animals are well fed they will grow rapidly and when they are not able to receive sufficient nutrients they will reduce their growth rate Recently it has been also demonstrated that cellular bicarbonate metabolism which is responsible for cell growth can be regulated by mTORC1 signaling 6 In addition the availability of amino acids to individual cells also directly promotes TOR activity although this mode of regulation is more important in single celled organisms than in multicellular organisms such as animals that always maintain an abundance of amino acids in circulation One disputed theory proposes that many different mammalian cells undergo size dependent transitions during the cell cycle These transitions are controlled by the cyclin dependent kinase Cdk1 7 Though the proteins that control Cdk1 are well understood their connection to mechanisms monitoring cell size remains elusive A postulated model for mammalian size control situates mass as the driving force of the cell cycle A cell is unable to grow to an abnormally large size because at a certain cell size or cell mass the S phase is initiated The S phase starts the sequence of events leading to mitosis and cytokinesis A cell is unable to get too small because the later cell cycle events such as S G2 and M are delayed until mass increases sufficiently to begin S phase 8 Cell populations editCell populations go through a particular type of exponential growth called doubling or cell proliferation Thus each generation of cells should be twice as numerous as the previous generation However the number of generations only gives a maximum figure as not all cells survive in each generation Cells can reproduce in the stage of Mitosis where they double and split into two genetically equal cells Cell size editCell size is highly variable among organisms with some algae such as Caulerpa taxifolia being a single cell several meters in length 9 Plant cells are much larger than animal cells and protists such as Paramecium can be 330 mm long while a typical human cell might be 10 mm How these cells decide how big they should be before dividing is an open question Chemical gradients are known to be partly responsible and it is hypothesized that mechanical stress detection by cytoskeletal structures is involved Work on the topic generally requires an organism whose cell cycle is well characterized Yeast cell size regulation edit The relationship between cell size and cell division has been extensively studied in yeast For some cells there is a mechanism by which cell division is not initiated until a cell has reached a certain size If the nutrient supply is restricted after time t 2 in the diagram below and the rate of increase in cell size is slowed the time period between cell divisions is increased 10 Yeast cell size mutants were isolated that begin cell division before reaching a normal regular size wee mutants 11 nbsp Figure 1 Cell cycle and growthWee1 protein is a tyrosine kinase that normally phosphorylates the Cdc2 cell cycle regulatory protein the homolog of CDK1 in humans a cyclin dependent kinase on a tyrosine residue Cdc2 drives entry into mitosis by phosphorylating a wide range of targets This covalent modification of the molecular structure of Cdc2 inhibits the enzymatic activity of Cdc2 and prevents cell division Wee1 acts to keep Cdc2 inactive during early G2 when cells are still small When cells have reached sufficient size during G2 the phosphatase Cdc25 removes the inhibitory phosphorylation and thus activates Cdc2 to allow mitotic entry A balance of Wee1 and Cdc25 activity with changes in cell size is coordinated by the mitotic entry control system It has been shown in Wee1 mutants cells with weakened Wee1 activity that Cdc2 becomes active when the cell is smaller Thus mitosis occurs before the yeast reach their normal size This suggests that cell division may be regulated in part by dilution of Wee1 protein in cells as they grow larger Linking Cdr2 to Wee1 edit The protein kinase Cdr2 which negatively regulates Wee1 and the Cdr2 related kinase Cdr1 which directly phosphorylates and inhibits Wee1 in vitro 12 are localized to a band of cortical nodes in the middle of interphase cells After entry into mitosis cytokinesis factors such as myosin II are recruited to similar nodes these nodes eventually condense to form the cytokinetic ring 13 A previously uncharacterized protein Blt1 was found to colocalize with Cdr2 in the medial interphase nodes Blt1 knockout cells had increased length at division which is consistent with a delay in mitotic entry This finding connects a physical location a band of cortical nodes with factors that have been shown to directly regulate mitotic entry namely Cdr1 Cdr2 and Blt1 Further experimentation with GFP tagged proteins and mutant proteins indicates that the medial cortical nodes are formed by the ordered Cdr2 dependent assembly of multiple interacting proteins during interphase Cdr2 is at the top of this hierarchy and works upstream of Cdr1 and Blt1 14 Mitosis is promoted by the negative regulation of Wee1 by Cdr2 It has also been shown that Cdr2 recruits Wee1 to the medial cortical node The mechanism of this recruitment has yet to be discovered A Cdr2 kinase mutant which is able to localize properly despite a loss of function in phosphorylation disrupts the recruitment of Wee1 to the medial cortex and delays entry into mitosis Thus Wee1 localizes with its inhibitory network which demonstrates that mitosis is controlled through Cdr2 dependent negative regulation of Wee1 at the medial cortical nodes 14 Cell polarity factors edit Cell polarity factors positioned at the cell tips provide spatial cues to limit Cdr2 distribution to the cell middle In fission yeast Schizosaccharomyces pombe S Pombe cells divide at a defined reproducible size during mitosis because of the regulated activity of Cdk1 15 The cell polarity protein kinase Pom1 a member of the dual specificity tyrosine phosphorylation regulated kinase DYRK family of kinases localizes to cell ends In Pom1 knockout cells Cdr2 was no longer restricted to the cell middle but was seen diffusely through half of the cell From this data it becomes apparent that Pom1 provides inhibitory signals that confine Cdr2 to the middle of the cell It has been further shown that Pom1 dependent signals lead to the phosphorylation of Cdr2 Pom1 knockout cells were also shown to divide at a smaller size than wild type which indicates a premature entry into mitosis 14 Pom1 forms polar gradients that peak at cell ends which shows a direct link between size control factors and a specific physical location in the cell 16 As a cell grows in size a gradient in Pom1 grows When cells are small Pom1 is spread diffusely throughout the cell body As the cell increases in size Pom1 concentration decreases in the middle and becomes concentrated at cell ends Small cells in early G2 which contain sufficient levels of Pom1 in the entirety of the cell have inactive Cdr2 and cannot enter mitosis It is not until the cells grow into late G2 when Pom1 is confined to the cell ends that Cdr2 in the medial cortical nodes is activated and able to start the inhibition of Wee1 This finding shows how cell size plays a direct role in regulating the start of mitosis In this model Pom1 acts as a molecular link between cell growth and mitotic entry through a Cdr2 Cdr1 Wee1 Cdk1 pathway 14 The Pom1 polar gradient successfully relays information about cell size and geometry to the Cdk1 regulatory system Through this gradient the cell ensures it has reached a defined sufficient size to enter mitosis Other experimental systems for the study of cell size regulation edit One common means to produce very large cells is by cell fusion to form syncytia For example very long several inches skeletal muscle cells are formed by fusion of thousands of myocytes Genetic studies of the fruit fly Drosophila have revealed several genes that are required for the formation of multinucleated muscle cells by fusion of myoblasts 17 Some of the key proteins are important for cell adhesion between myocytes and some are involved in adhesion dependent cell to cell signal transduction that allows for a cascade of cell fusion events Increases in the size of plant cells are complicated by the fact that almost all plant cells are inside of a solid cell wall Under the influence of certain plant hormones the cell wall can be remodeled allowing for increases in cell size that are important for the growth of some plant tissues Most unicellular organisms are microscopic in size but there are some giant bacteria and protozoa that are visible to the naked eye See Table of cell sizes Dense populations of a giant sulfur bacterium in Namibian shelf sediments 18 Large protists of the genus Chaos closely related to the genus Amoeba In the rod shaped bacteria E coli Caulobacter crescentus and B subtilis cell size is controlled by a simple mechanisms in which cell division occurs after a constant volume has been added since the previous division 19 20 By always growing by the same amount cells born smaller or larger than average naturally converge to an average size equivalent to the amount added during each generation Cell division editCell reproduction is asexual For most of the constituents of the cell growth is a steady continuous process interrupted only briefly at M phase when the nucleus and then the cell divide in two The process of cell division called cell cycle has four major parts called phases The first part called G1 phase is marked by synthesis of various enzymes that are required for DNA replication The second part of the cell cycle is the S phase where DNA replication produces two identical sets of chromosomes The third part is the G2 phase in which a significant protein synthesis occurs mainly involving the production of microtubules that are required during the process of division called mitosis The fourth phase M phase consists of nuclear division karyokinesis and cytoplasmic division cytokinesis accompanied by the formation of a new cell membrane This is the physical division of mother and daughter cells The M phase has been broken down into several distinct phases sequentially known as prophase prometaphase metaphase anaphase and telophase leading to cytokinesis Cell division is more complex in eukaryotes than in other organisms Prokaryotic cells such as bacterial cells reproduce by binary fission a process that includes DNA replication chromosome segregation and cytokinesis Eukaryotic cell division either involves mitosis or a more complex process called meiosis Mitosis and meiosis are sometimes called the two nuclear division processes Binary fission is similar to eukaryote cell reproduction that involves mitosis Both lead to the production of two daughter cells with the same number of chromosomes as the parental cell Meiosis is used for a special cell reproduction process of diploid organisms It produces four special daughter cells gametes which have half the normal cellular amount of DNA A male and a female gamete can then combine to produce a zygote a cell which again has the normal amount of chromosomes The rest of this article is a comparison of the main features of the three types of cell reproduction that either involve binary fission mitosis or meiosis The diagram below depicts the similarities and differences of these three types of cell reproduction nbsp Cell growthComparison of the three types of cell division edit The DNA content of a cell is duplicated at the start of the cell reproduction process Prior to DNA replication the DNA content of a cell can be represented as the amount Z the cell has Z chromosomes After the DNA replication process the amount of DNA in the cell is 2Z multiplication 2 x Z 2Z During Binary fission and mitosis the duplicated DNA content of the reproducing parental cell is separated into two equal halves that are destined to end up in the two daughter cells The final part of the cell reproduction process is cell division when daughter cells physically split apart from a parental cell During meiosis there are two cell division steps that together produce the four daughter cells After the completion of binary fission or cell reproduction involving mitosis each daughter cell has the same amount of DNA Z as what the parental cell had before it replicated its DNA These two types of cell reproduction produced two daughter cells that have the same number of chromosomes as the parental cell Chromosomes duplicate prior to cell division when forming new skin cells for reproduction After meiotic cell reproduction the four daughter cells have half the number of chromosomes that the parental cell originally had This is the haploid amount of DNA often symbolized as N Meiosis is used by diploid organisms to produce haploid gametes In a diploid organism such as the human organism most cells of the body have the diploid amount of DNA 2N Using this notation for counting chromosomes we say that human somatic cells have 46 chromosomes 2N 46 while human sperm and eggs have 23 chromosomes N 23 Humans have 23 distinct types of chromosomes the 22 autosomes and the special category of sex chromosomes There are two distinct sex chromosomes the X chromosome and the Y chromosome A diploid human cell has 23 chromosomes from that person s father and 23 from the mother That is your body has two copies of human chromosome number 2 one from each of your parents nbsp ChromosomesImmediately after DNA replication a human cell will have 46 double chromosomes In each double chromosome there are two copies of that chromosome s DNA molecule During mitosis the double chromosomes are split to produce 92 single chromosomes half of which go into each daughter cell During meiosis there are two chromosome separation steps which assure that each of the four daughter cells gets one copy of each of the 23 types of chromosome Sexual reproduction edit Main article Evolution of sex Further information Origin and function of meiosis and Homologous recombination Though cell reproduction that uses mitosis can reproduce eukaryotic cells eukaryotes bother with the more complicated process of meiosis because sexual reproduction such as meiosis confers a selective advantage Notice that when meiosis starts the two copies of sister chromatids number 2 are adjacent to each other During this time there can be genetic recombination events Information from the chromosome 2 DNA gained from one parent red will transfer over to the chromosome 2 DNA molecule that was received from the other parent green Notice that in mitosis the two copies of chromosome number 2 do not interact Recombination of genetic information between homologous chromosomes during meiosis is a process for repairing DNA damages This process can also produce new combinations of genes some of which may be adaptively beneficial and influence the course of evolution However in organisms with more than one set of chromosomes at the main life cycle stage sex may also provide an advantage because under random mating it produces homozygotes and heterozygotes according to the Hardy Weinberg ratio Disorders editA series of growth disorders can occur at the cellular level and these consequently underpin much of the subsequent course in cancer in which a group of cells display uncontrolled growth and division beyond the normal limits invasion intrusion on and destruction of adjacent tissues and sometimes metastasis spread to other locations in the body via lymph or blood Several key determinants of cell growth like ploidy and the regulation of cellular metabolism are commonly disrupted in tumors 21 Therefore heterogenous cell growth and pleomorphism is one of the earliest hallmarks of cancer progression 22 23 Despite the prevalence of pleomorphism in human pathology its role in disease progression is unclear In epithelial tissues misregulation of cellular size can induce packing defects and disperse aberrant cells 24 But the consequence of atypical cell growth in other animal tissues is unknown Measurement methods editThe cell growth can be detected by a variety of methods The cell size growth can be visualized by microscopy using suitable stains But the increase of cells number is usually more significant It can be measured by manual counting of cells under microscopy observation using the dye exclusion method i e trypan blue to count only viable cells Less fastidious scalable methods include the use of cytometers while flow cytometry allows combining cell counts events with other specific parameters fluorescent probes for membranes cytoplasm or nuclei allow distinguishing dead viable cells cell types cell differentiation expression of a biomarker such as Ki67 Beside the increasing number of cells one can be assessed regarding the metabolic activity growth that is the CFDA and calcein AM measure fluorimetrically not only the membrane functionality dye retention but also the functionality of cytoplasmic enzymes esterases The MTT assays colorimetric and the resazurin assay fluorimetric dose the mitochondrial redox potential All these assays may correlate well or not depending on cell growth conditions and desired aspects activity proliferation The task is even more complicated with populations of different cells furthermore when combining cell growth interferences or toxicity See also editBacterial growthReferences edit a b c Conlon Ian Raff Martin 1999 Size Control in Animal Development Cell 96 2 235 244 doi 10 1016 S0092 8674 00 80563 2 ISSN 0092 8674 PMID 9988218 S2CID 15738174 Grewal Savraj S Edgar Bruce A 2003 Controlling cell division in yeast and animals does size matter Journal of Biology 2 1 5 doi 10 1186 1475 4924 2 5 ISSN 1475 4924 PMC 156596 PMID 12733996 Neufeld Thomas P de la Cruz Aida Flor A Johnston Laura A Edgar Bruce A 1998 Coordination of Growth and Cell Division in the Drosophila Wing Cell 93 7 1183 1193 doi 10 1016 S0092 8674 00 81462 2 ISSN 0092 8674 PMID 9657151 S2CID 14608744 Thompson Barry J 2010 Developmental control of cell growth and division in Drosophila Current Opinion in Cell Biology 22 6 788 794 doi 10 1016 j ceb 2010 08 018 PMID 20833011 Hafen E 2004 Interplay Between Growth Factor and Nutrient Signaling Lessons from Drosophila TOR TOR Current Topics in Microbiology and Immunology Vol 279 pp 153 167 doi 10 1007 978 3 642 18930 2 10 ISBN 978 3 642 62360 8 ISSN 0070 217X PMID 14560957 Ali E Liponska A O Hara B Amici D Torno M Gao P Asara J Yap M N F Mendillo M Ben Sahra I June 2022 The mTORC1 SLC4A7 axis stimulates bicarbonate import to enhance de novo nucleotide synthesis Molecular Cell 82 1 3284 3298 e7 doi 10 1016 j molcel 2022 06 008 PMC 9444906 PMID 35772404 Mitchison JM 2003 Growth during the cell cycle Int Rev Cytol International Review of Cytology 226 165 258 doi 10 1016 S0074 7696 03 01004 0 ISBN 978 0 12 364630 9 PMID 12921238 Cooper Stephen 2004 Control and maintenance of mammalian cell size BMC Cell Biology 5 1 35 doi 10 1186 1471 2121 5 35 PMC 524481 PMID 15456512 Peplow Mark 23 March 2005 Algae create glue to repair cell damage Nature com Retrieved 4 July 2016 Slavov N Botstein D June 2011 Coupling among Growth Rate Response Metabolic Cycle and Cell Division Cycle in Yeast Molecular Biology of the Cell 22 12 1997 2009 doi 10 1091 mbc E11 02 0132 PMC 3113766 PMID 21525243 Wee1 mutants of S pombe have small cell size and the homologous proteins in humans also regulate cell entry into mitosis in Lodish HF Berk A Zipursky LS Matsudaira P et al eds 2000 Molecular cell biology 4th ed New York W H Freeman ISBN 978 0 7167 3136 8 Wu L Russell P June 1993 Nim1 kinase promotes mitosis by inactivating Wee1 tyrosine kinase Nature 363 6431 738 41 Bibcode 1993Natur 363 738W doi 10 1038 363738a0 PMID 8515818 S2CID 4320080 Wu JQ Kuhn JR Kovar DR Pollard TD November 2003 Spatial and temporal pathway for assembly and constriction of the contractile ring in fission yeast cytokinesis Dev Cell 5 5 723 34 doi 10 1016 S1534 5807 03 00324 1 PMID 14602073 a b c d Moseley JB Mayeux A Paoletti A Nurse P June 2009 A spatial gradient coordinates cell size and mitotic entry in fission yeast Nature 459 7248 857 60 Bibcode 2009Natur 459 857M doi 10 1038 nature08074 PMID 19474789 S2CID 4330336 Rupes I September 2002 Checking cell size in yeast Trends Genet 18 9 479 85 doi 10 1016 S0168 9525 02 02745 2 PMID 12175809 Padte NN Martin SG Howard M Chang F December 2006 The cell end factor pom1p inhibits mid1p in specification of the cell division plane in fission yeast Curr Biol 16 24 2480 7 doi 10 1016 j cub 2006 11 024 PMID 17140794 Menon SD Osman Z Chenchill K Chia W June 2005 A positive feedback loop between Dumbfounded and Rolling pebbles leads to myotube enlargement in Drosophila J Cell Biol 169 6 909 20 doi 10 1083 jcb 200501126 PMC 2171639 PMID 15955848 Schulz HN Brinkhoff T Ferdelman TG Marine MH Teske A Jorgensen BB April 1999 Dense populations of a giant sulfur bacterium in Namibian shelf sediments Science 284 5413 493 5 Bibcode 1999Sci 284 493S doi 10 1126 science 284 5413 493 PMID 10205058 S2CID 32571118 Taheri Araghi S Bradde S Sauls J T Hill N S Levin P A Paulsson J Vergassola M Jun S February 2015 Cell size control and homeostasis in bacteria Current Biology 25 3 385 391 doi 10 1016 j cub 2014 12 009 PMC 4323405 PMID 25544609 Campos M Surovtsev I V Kato S Paintdakhi A Beltran B Ebmeier S E Jacobs Wagner C December 2014 A constant size extension drives bacterial cell size homeostasis Cell 159 6 1433 1446 doi 10 1016 j cell 2014 11 022 PMC 4258233 PMID 25480302 Schmoller Kurt M Skotheim Jan M December 2015 The Biosynthetic Basis of Cell Size Control Trends Cell Biol 25 12 793 802 doi 10 1016 j tcb 2015 10 006 PMC 6773270 PMID 26573465 Travis W D Brambilla B Burke A P Marx A Nicholson A G 2015 WHO Classification of Tumours of the Lung Pleura Thymus and Heart Lyon International Agency for Research on Cancer ISBN 978 92 832 2436 5 El Naggar A K Chan J C K Grandis J R Takata T Slootweg P J 2017 01 23 WHO Classification of Head and Neck Tumours Lyon International Agency for Research on Cancer also known as Adman ISBN 978 92 832 2438 9 Archived from the original on 2019 10 31 Retrieved 2019 10 31 Ramanathan Subramanian P Krajnc Matej Gibson Matthew C October 2019 Cell Size Pleomorphism Drives Aberrant Clone Dispersal in Proliferating Epithelia Developmental Cell 51 1 49 61 e4 doi 10 1016 j devcel 2019 08 005 PMC 6903429 PMID 31495693 Books editMorgan David O 2007 The cell cycle principles of control London Sunderland Mass ISBN 978 0 9539181 2 6 External links editA comparison of generational and exponential models of cell population growth Local Growth in an Array of Disks Wolfram Demonstrations Project Retrieved from https en wikipedia org w index php title Cell growth amp oldid 1193655704, wikipedia, wiki, book, books, library,

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