Studies on the permeability of rat liver lysosomes to carbohydrates

Lloyd, John

doi:10.1042/bj1150703

Cited by 70 publications

(35 citation statements)

References 17 publications

(8 reference statements)

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“…In conclusion it is hypothesized that sorbitol uptake in glial primary cultures is mediated by a simple diffusion mechanism through a pore-like protein structure embedded in the lipid bilayer. Chromaffin granules from bovine adrenal glands are permeable to a variety of hexitols, whereas rat liver lysosomes apparently do not take up these compounds (Lloyd, 1969;Perlman, 1976). Therefore uptake of sorbitol may also be a particular property of the cells constituting the astrogliarich primary culture and is not in contrast to the postulated lack of permeability of sorbitol in cells of the peripheral nervous system (Cohen, 1987).…”

Section: Discussionmentioning

confidence: 99%

Characteristics of Sorbitol Uptake in Rat Glial Primary Cultures

Stahl

Wiesinger

Hamprecht

1989

Journal of Neurochemistry

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Uptake of [U-14C]sorbitol was studied in astrogliarich rat primary cultures. Initial rate of sorbitol uptake is proportional to sorbitol concentration between 20 microM and 400 mM. Sorbitol transport is not inhibited by glucose, fructose, and a variety of structurally related polyols, or by cytochalasin B, an inhibitor of glucose transport. Phloretin, phlorizin, filipin, and n-hexanol, all compounds that alter the properties of biological membranes, and the sulfhydryl reagent p-chloromercuribenzoate inhibit sorbitol uptake to various degrees. Variation in the concentrations of extracellular Na+ and K+ does not affect transfer of sorbitol across the cell membrane. It is concluded that sorbitol is taken up into glial cells by a diffusion process, not involving a carrier and probably not through the lipid bilayer, but through a proteinaceous channel-like structure.

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Section: Discussionmentioning

confidence: 99%

Characteristics of Sorbitol Uptake in Rat Glial Primary Cultures

Stahl

Wiesinger

Hamprecht

1989

Journal of Neurochemistry

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“…Other lysosomal enzymes, including ␣ -fucosidase, ␣ -mannosidase and ␤ -N-acetylglucosaminidase, have also been reported in bovine RPE [119] . Natural macromolecular drugs as well as xenobiotics may be degraded by lysosomal enzymes during transport across the RPE, as they are able to cross lysosomal membranes by passive diffusion [120,121] .…”

Section: Cytochrome P-450mentioning

confidence: 99%

Transport Barriers in Transscleral Drug Delivery for Retinal Diseases

et al. 2007

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Transscleral delivery has emerged as an attractive method for treating retinal disorders because it offers localized delivery of drugs as a less invasive method compared to intravitreal administration. Numerous novel transscleral drug delivery systems ranging from microparticles to implants have been reported. However, transscleral delivery is currently not as clinically effective as intravitreal delivery in the treatment of retinal diseases. Transscleral drug delivery systems require drugs to permeate through several layers of ocular tissue (sclera, Bruch’s membrane-choroid, retinal pigment epithelium) to reach the neuroretina. As a result, a steep drug concentration gradient from the sclera to the retina is established, and very low concentrations of drug are detected in the retina. This steep gradient is created by the barriers to transport that hinder drug molecules from successfully reaching the retina. A review of the literature reveals 3 types of barriers hindering transscleral drug delivery: static, dynamic and metabolic. While static barriers have been examined in detail, the literature on dynamic and metabolic barriers is lacking. These barriers must be investigated further to gain a more complete understanding of the transport barriers involved in transscleral drug delivery.

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“…Relative permeabilities of the membrane to different solutes have been measured (Lloyd, 1969(Lloyd, , 1971Lee, 1970Lee, , 1971, by suspending the lysosomes in iso-osmotic solutions of different solutes and measuring the release of soluble enzymes, as an index of lysis.…”

Section: Permeability Ofprimary Granule Fraction To Different Compoundsmentioning

confidence: 99%

Progesterone-induced lysis of rat kidney lysosomes as studied by changes in light-absorbance

Badenoch‐Jones¹,

Baum²

1974

Biochemical Journal

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1. A rat kidney lysosomal fraction was prepared by the method of Maunsbach (1966) and characterized by its content of representative marker enzymes for lysosomes, mitochondria, peroxisomes and endoplasmic reticulum. 2. It was shown that both pHdependent and progesterone-induced lysis lead to a decrease in the E520 of suspensions of this preparation. This decrease parallels quantitatively and temporally the release of soluble acid phosphatase. 3. It is suggested that E520 measurements are a valid method for the continuous measurement of changes in lysosomal integrity. 4. As an example, results are included which demonstrate the ability of Zn2+ to stabilize lysosomes against spontaneous and progesterone-induced lysis.

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Studies on the permeability of rat liver lysosomes to carbohydrates

Cited by 70 publications

References 17 publications

Characteristics of Sorbitol Uptake in Rat Glial Primary Cultures

Characteristics of Sorbitol Uptake in Rat Glial Primary Cultures

Transport Barriers in Transscleral Drug Delivery for Retinal Diseases

Progesterone-induced lysis of rat kidney lysosomes as studied by changes in light-absorbance

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