Changes in insulin-receptor structure associated with trypsin-induced activation of the receptor tyrosine kinase

Clark, Stella; Eckardt, Glenn S.; Siddle, Kenneth; Harrison, Len C.

doi:10.1042/bj2760027

Cited by 24 publications

(29 citation statements)

References 29 publications

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“…This discrepancy may be largely due to di erent experimental procedures: in the previous report, cells were trypsinized and then kept in suspension for 30 min. In our experiments, cells were detached by Versene, since, as mentioned above, trypsinization is known to partially digest the extracellular portions of growth factor receptors (Clark et al, 1991). Also at variance with other experimental situations, we found a lack of correlation with the serine/threonine kinase Akt, activation which has also been shown to be important in protection from apoptosis, including IGF-I mediated protection (Kennedy et al, 1997;Khwaja et al, 1997;Datta et al, 1997).…”

Section: Discussionmentioning

confidence: 59%

“…In preliminary experiments (not shown), we had observed that detachment of cells by trypsinization (as it is usually done also in our laboratory) caused the results to be somewhat erratic, probably due to the fact that trypsinization, even modest, induces partial breakdown of the extracellular part of growth factor receptors (Clark et al, 1991). p6 cells (mouse embryo ®broblasts that over-express the human IGF-IR) were chosen for the initial experiments, because they are known to form colonies in soft agar very e ciently (Pietrzkowski et al, 1992), and to grow in anchorageindependent conditions in vivo .…”

Section: Resultsmentioning

confidence: 78%

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Anti-apoptotic signaling of the IGF-I receptor in fibroblasts following loss of matrix adhesion

et al. 1999

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The type 1 insulin-like growth factor receptor (IGF-IR) is known to protect cells from a variety of apoptotic injuries. In several instances, the anti-apoptotic e ect of the wild type IGF-IR is more evident under conditions of anchorage-independence than in cells in monolayer cultures. We have investigated IGF-IR signaling in cells in anoikis, a form of apoptosis that occurs when cells are denied attachment to the extra-cellular matrix. IGF-I protects mouse embryo ®broblasts (MEF) from anoikis caused by withdrawal of growth factors. Survival is dependent on the concentration of IGF-I and a su cient number of functional IGF-I receptors. In this model, IGF-I protection correlates best with ras activation and cell-to-cell aggregation, while PI3-kinase, Akt and MAP kinases seem to play a lesser, alternative role.

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Section: Discussionmentioning

confidence: 59%

Section: Resultsmentioning

confidence: 78%

Anti-apoptotic signaling of the IGF-I receptor in fibroblasts following loss of matrix adhesion

et al. 1999

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“…As reported by other investigators, only receptors exposed to the extracellular medium are accessible to trypsin [4,23 26]. This treatment proteolyzes the ~-subunit of the receptor in a unique site close to the C-terminus of the ~-subunit and separates both subunits [27]. The larger fragment resulting from this treatment (100 kDa) contains both the mAb 83-7 and insulin binding sites, whereas the smaller fragment remains attached to the fl-subunit of the receptor [27].…”

Section: Resultsmentioning

confidence: 80%

“…These antibodies have been extensively described by Clark et al [27]. Anti-phosphotyrosine antibody 4GI0 was purchased from Upstate Biotechnologies.…”

Section: Methodsmentioning

confidence: 99%

“…Internalized receptors were distinguished from those present on the cell surface on the basis of their sensitivity to mild trypsin treatment of the cells, as originally described by Levy and Olefsky [24], a procedure that has been used as a tool to distinguish cell surface from internalized receptors [4,[23][24][25][26]. Mild trypsin treatment (1 mg/ml trypsin for 30 min at 4°C) cleaves the ~-subunit of the receptor predominantly at one site, releasing two fragments: a 100 kDa fragment that contains the binding sites for insulin and for the monoclonal antibody 83-7, and a 20 kDa fragment that remains attached to the fl-subunit [27]. Thus, the criterion used to detect intact receptors was the co-immunoprecipitation of c~-and fl-subunits: only those fl-subunits attached to intact, non-proteolyzed c~-subunits coimmunoprecipitate with mAb 83-7.…”

Section: Redistribution Of the Insulin Receptormentioning

confidence: 99%

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Brefeldin A inhibits insulin‐dependent receptor redistribution in HIRcB cells

Shome

Romero

1995

FEBS Letters

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Brefeldin A (BFA) is a potent inhibitor of intracellular vesicle traffic. We have investigated the effects of BFA on the traffic of the insulin receptor in HIRcB cells, a cell line derived from Rat-1 fibroblasts that over-expresses a normal human insulin receptor. We report here that insulin-dependent receptor redistribution is inhibited by BFA and that this drug has no effects on the insulin-independent redistribution of the receptor. Autophosphorylation of the insulin receptor and the stimulation of mitogen-activated protein kinase (MAPK) by insulin were not affected by treatment with the drug. The effects of BFA were further shown to require addition of the drug prior to the addition of insulin. BFA added 10 rain after stimulation with insulin had no effects on the redistribution of the receptor. Dose-response studies demonstrated that the effects of BFA were half-maximal at a dose of 1 ttglml and maximal at about 10 pg/ml. These findings suggest that BFA blocks an early step in the chain of events that lead to insulin receptor internalization without affecting the interactions of the receptor with insulin, the stimulation of the tyrosine kinase activity of the receptor by the hormone, or other insulin-regulated signalling pathways, such as the activation of MAPK.

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Insulin-like growth factor-I-mediated survival from Anoikis: Role of cell aggregation and focal adhesion kinase

1998

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Anoikis is a form of cell death that occurs when cells are denied attachment to the extra-cellular matrix. Using p6 cells, that are 3T3 cells overexpressing the type 1 insulin-like growth factor receptor (IGF-IR), we show that these cells undergo apoptosis when seeded on polyHEMA plates in serum-free medium (SFM). IGF-I protects p6 cells from anoikis, without inducing mitogenesis or DNA synthesis. In the surviving p6 cells in suspension cultures, the focal adhesion kinase (FAK) is tyrosyl phosphorylated by IGF-I, although this phosphorylation occurs only after several hours. The importance of FAK in protection from anoikis is confirmed by v-src-transformed R-cells, in which FAK is constitutively phosphorylated, that survive even in SFM. Surviving cells, whether p6 or v-src transformed, tend to form large cell aggregates, whose appearance precedes the phosphorylation of FAK. These and other findings suggest that FAK phosphorylation in the case of IGF-I is a mediated effect rather than a direct one. When p6 cells are plated on polyHEMA dishes, IGF-I induces cell aggregation and this aggregation correlates with survival and the eventual phosphorylation of FAK.

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Changes in insulin-receptor structure associated with trypsin-induced activation of the receptor tyrosine kinase

Cited by 24 publications

References 29 publications

Anti-apoptotic signaling of the IGF-I receptor in fibroblasts following loss of matrix adhesion

Anti-apoptotic signaling of the IGF-I receptor in fibroblasts following loss of matrix adhesion

Brefeldin A inhibits insulin‐dependent receptor redistribution in HIRcB cells

Insulin-like growth factor-I-mediated survival from Anoikis: Role of cell aggregation and focal adhesion kinase

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