Gene/Protein
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Drug
Enzyme
Compound
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Gene/Protein
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Drug
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Target Concepts:
Gene/Protein
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Query: EC:4.1.99.3 (
PRE
)
1,923
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Using light and electron microscopy, we have confirmed an earlier observation that chick embryonic pigmented retina epithelial cells (
PRE
cells) seeded in vitro on cultured sheets of choroid fibroblasts, are able to spread. Spreading is as rapid (and shows the same dependence on lateral contact between
PRE
cells) as on a serum-coated culture substrate. After 1 h most cells are spreading on the upper surface of the choroid sheet, but after 4 h, some
PRE
cells can be found sandwiched between overlapping choroid cells, and thus have invaded the sheet.
Choroid
fibroblasts underlie
PRE
in vivo, but the ability of
PRE
cells to spread on cultured fibroblasts is not specific for choroid, since
PRE
cells spread also on BKH21 hamster kidney fibroblasts, and on fibroblasts from chick embryonic heart. As reported by others for various fibroblastic cells, choroid cells seeded on to choroid sheets or on to cultured
PRE
are unable to spread. A possible explanation is that spreading of adherent cells is contact-inhibited by the cells in the sheet, just as their leading edges are paralysed on contact, and thus locomotion is inhibited, when fibroblasts collide on a plane substratum. If spreading of seeded cells and cell locomotion are inhibited by the same mechanism,
PRE
cells should contact-inhibit choroid fibroblasts with which they collide, but not themselves be so inhibited. Using time-lapse cinemicrography, we have found this to be the case. We first established that in homotypic collisions, choroid fibroblasts do show contact inhibition of locomotion, despite the criss-cross (not well monolayered) appearance of confluent cultures. In heterotypic collisions between choroid and
PRE
we found the predicted nonreciprocal behaviour: the choroid leading edge is paralysed on collision, and the cell subsequently retracts, whereas the active
PRE
margin appears to be completely unaffected. Speed measurements from a series of such collisions show that the speed of choroid cells is markedly reduced on collision with
PRE
, whereas the slight slowing of
PRE
is not statistically significant. We have observed similar behaviour in heterotypic collisions between various epithelial and fibroblastic cells, and so it seems possible that non-reciprocity may prove general for this interaction. If so, it has important implications for the role of contact inhibition of locomotion in phenomena such as morphogenesis, wound healing and the invasiveness of carcinoma cells. On the one hand, non-reciprocal contact-inhibition of locomotion may permit the spreading of epithelia over mesenchymal cells, thus generating or restoring an epithelial bounding membrane. On the other hand, in the absence of other interactions, it would fail to inhibit the invasion of mesenchymal territory by aberrant epithelial cells, or presumably by epithelial free edges.
...
PMID:Non-reciprocal contact inhibition of locomotion of chick embryonic choroid fibroblasts by pigmented retina epithelial cells. 72 99
A pharmacokinetic study is described in which Friesian calves (n = 30) were treated orally with clenbuterol at 10 times the therapeutic dose. The study was designed to establish the distribution and elimination of clenbuterol from edible tissues, the major compartments of the eye and body fluids. Animals (n = 24) were dosed (10 micrograms/kg body weight) twice daily with clenbuterol for 21 days and slaughtered in groups of five (one untreated control animal per group) at 6 h and 1, 2, 4, 8 and 16 days after cessation of treatment. At slaughter, samples of diaphragm muscle, liver, kidney, bile, urine and both eyes were obtained. One of the eyes was separated into constituent tissues: aqueous humour, vitreous humour, cornea, lens, retina (without pigmented epithelium), choroid (with pigmented retinal epithelium; choroid/
PRE
) and sclera. All samples were stored at -20 degrees C. Clenbuterol concentrations were higher in liver than kidney, bile and urine from day 2 of withdrawal onwards. Concentrations in choroid/
PRE
were at least 10 times higher than in liver at all periods following cessation of treatment and 52 times higher 16 days after treatment. The concentrations of clenbuterol in the constituent tissues of the eye were in the order choroid/
PRE
> cornea > > retina > aqueous humour/vitreous humour > or = lens. Concentrations of clenbuterol in choroid/
PRE
taken from eyes frozen whole were generally lower than those in choroid/
PRE
separated before storage.
Choroid
/
PRE
stored by either method contained clenbuterol at more than 100 ng/g 16 days following cessation of treatment.(ABSTRACT TRUNCATED AT 250 WORDS)
...
PMID:Distribution and elimination of clenbuterol in tissues and fluids of calves following prolonged oral administration at a growth-promoting dose. 762 33
