2006
DOI: 10.7150/ijbs.2.216
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Homeostatic restitution of cell membranes. Nuclear membrane lipid biogenesis and transport of protein from cytosol to intranuclear spaces.

Abstract: Our studies on homeostatic restitution of cellular and subcellular membranes showed that vesicular intracellular transport is engaged in systematic and coordinated replacement of lipids and proteins in the membranes of the secretory, non-dividing epithelial cells (Slomiany et al., J. Physiol. Pharmacol. 2004; 55: 837-860). In this report, we present evidence on the homeostatic restitution of lipids in the biomembranes that constitute nuclear envelopes. We investigated nuclear membranes lipid synthesis by emplo… Show more

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Cited by 9 publications
(57 citation statements)
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References 37 publications
(95 reference statements)
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“…And, in the same construal of the metabolic cycle, the products of endocytosis, distinguished by their SM placement, are reflecting the composition of apical or basolateral membranes and are recognizable as genuine cell membrane-derived autophagocytes which are destined for the engulfment by lysosomal membrane and intralysosomal degradation. In keeping with our results-driven conclusions that all cell membranes are in continuous cycle of synthesis, replacement and degradation, the speculation with regard of the restitution of the ER and Golgi, the organelles most heavily involved in synthesis, modification, and trafficking of protein, is eminent but not through reprocessing of transport vesicles [14] As found out in the case of ER, the part of membrane adjacent to nuclear contents provides the link between nuclear pores, and as demonstrated with nuclear turnover of phosphoinositides, is in a constant lateral motion transporting cytosolic proteins to the nucleus, while in the same membrane, the lipids' synthesis-propelling motion delivers RNAs to cytosol [40] [41]. The reemerging from nucleus membrane must serve as the initial template that signals the translation of just produced and released mRNA and the integration of the product within co-synthesized organelle and/or membrane-specific lipids.…”
Section: Discussionmentioning
confidence: 99%
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“…And, in the same construal of the metabolic cycle, the products of endocytosis, distinguished by their SM placement, are reflecting the composition of apical or basolateral membranes and are recognizable as genuine cell membrane-derived autophagocytes which are destined for the engulfment by lysosomal membrane and intralysosomal degradation. In keeping with our results-driven conclusions that all cell membranes are in continuous cycle of synthesis, replacement and degradation, the speculation with regard of the restitution of the ER and Golgi, the organelles most heavily involved in synthesis, modification, and trafficking of protein, is eminent but not through reprocessing of transport vesicles [14] As found out in the case of ER, the part of membrane adjacent to nuclear contents provides the link between nuclear pores, and as demonstrated with nuclear turnover of phosphoinositides, is in a constant lateral motion transporting cytosolic proteins to the nucleus, while in the same membrane, the lipids' synthesis-propelling motion delivers RNAs to cytosol [40] [41]. The reemerging from nucleus membrane must serve as the initial template that signals the translation of just produced and released mRNA and the integration of the product within co-synthesized organelle and/or membrane-specific lipids.…”
Section: Discussionmentioning
confidence: 99%
“…The cells were prepared from rat gastric mucosa and the liver as described previously [41] [46]- [50]. The single cells that were separated from larger debris with the aid of specific cell size nylon mesh, were centrifuged at 50 xg for 2 min, washed twice with the enzyme-free medium, twice with the Minimum Essential Medium (MEM), and counted in hemocytometer.…”
Section: Preparation Of Cells For Subcellular Fractionationmentioning
confidence: 99%
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“…The carefully separated nuclei from cell organelles and the cell cytosol were subjected to treatments described earlier that affords mixture of membrane fragments commonly identified as outer and inner nuclear membranes (ONM, INM) [34]. To separate them into distinct fractions, the preparation of purified nuclear pellet recovered after centrifugation at 27,000 rpm in Beckman 45 Ti rotor for 1h was suspended at concentration of 2 mg protein/ml in a buffer consisting of 50 mM TIS-HCl pH 7.4, 0.25 M sucrose, 10 mM MgCl 2 , 1 mM DTT, 10 mg/ml leupeptin and 2 mM PMSF and then adjusted to 1% (w/v) with sodium citrate.…”
Section: Preparation Of Outer and Inner Nuclear Membranesmentioning
confidence: 99%