Dimensional regulation of cell-cycle events in Escherichia coli during steady-state growth

Grover, N.B.; Woldringh, Conrad L.

doi:10.1099/00221287-147-1-171

Cited by 35 publications

(34 citation statements)

References 21 publications

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“…Growth of E. coli occurs by the periodic succession of elongation and division events (1,2). Cells divide at their midpoint once the chromosome is replicated and the initial length is doubled (8). Cellular morphology is remarkably constant, and observation of aberrant shapes is extremely rare.…”

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confidence: 99%

Branching of Escherichia coli Cells Arises from Multiple Sites of Inert Peptidoglycan

et al. 2003

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Some strains of Escherichia coli defective for dacA, the gene coding for penicillin-binding protein 5, exhibit a strong branching phenotype when cell division is blocked. Since such branch formation implies a differentiation of polar caps at ectopic locations in the cell envelope, we analyzed murein segregation and observed a strong correlation between areas of inert murein and these morphological anomalies. In particular, the tips of branches exhibited the same properties as those described for polar caps of wild-type cells, i.e., the synthesis and turnover of murein were inhibited. Also, the mobility of cell envelope proteins was apparently constrained in areas with morphological defects. Polar regions of branching cells and sacculi had aberrant morphologies with a very high frequency. Of special interest was that areas of inert murein at polar caps were often split by areas of active synthesis, a situation unlike that observed in wild-type cells. These observations suggest that in dacA mutants, branches and other morphological anomalies may arise from split polar caps or by de novo generation of new poles built around inert peptidoglycan patches in the side walls of the cell.

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confidence: 99%

Branching of Escherichia coli Cells Arises from Multiple Sites of Inert Peptidoglycan

et al. 2003

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“…2b. The RVI mechanisms of astrocytes are also recognized as influx of Na 4 , K, and 2C1 by co-transporters and uptake of organic osmolyte through Na 4 concentration regulated channels [ 12]. Upon switching back to isotonic solution after RVI, we observed a significant secondary RVD (see fig.…”

Section: Cell Volume Response To Anisotonic Stimulimentioning

confidence: 78%

“…It is possible to use the kinetic response of cell volume as an indicator to achieve a cell based screen. There are a variety of methods to measure cell volume, which include confocal microscopy, electron microscopy [4,5], laser scattering, fluorescence intensity measurement [6,7], Coulter counter [8], and other electrical impedance measurements [9]. However, most methods to measure cell volume are time consuming, and either lack-resolution or require complex apparatus.…”

Section: Introductionmentioning

confidence: 99%

Microfluidic Cell Volume Biosensor for High Throughput Drug Screening

2004

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The maintenance of cell volume is critical to health. Cell volume change reflects many biological and physiological processes. We have developed a lab-chip to measure cell volume change in real-time with high sensitivity and resolution, and applicable to both adherent and suspended cell populations. The volume change was detected by measuring the impedance of extra-cellular solution within a microfluidic chamber containing the cells. Using microfabrication to make precise chamber dimensions, volume change can be detected in response to an osmotic gradient

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“…Unfortunately, the Pearson type III distribution does not allow the incorporation of such a relationship and consequently this feature is absent from the current model*a limitation we have not been able to overcome. But the normal (and hence reciprocal-normal) distribution does (Grover & Woldringh, 2001), quite easily.…”

Section: Discussionmentioning

confidence: 96%