Monoclonal antibodies reacting with multiple epitopes on the human insulin receptor

Soos, Maria A.; Siddle, Kenneth; Baron, Michael D.; Heward, JM; Luzio, J. Paul; Bellatin, Jaime; Lennox, Edwin S.

doi:10.1042/bj2350199

Cited by 195 publications

(187 citation statements)

References 45 publications

(41 reference statements)

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“…Cell-surface expression was monitored by FACS analysis with mAb 83.7 [39]. All except one of the stable cell lines showed increases in fluorescence of more than 18-fold that of the parental CHO-K1 cell line ( Figure 2) and comparable with that of the CHO.T cell line (Table 1), which produces more than 250 000 insulin receptors per cell [34].…”

Section: Whole Hir Mutantsmentioning

confidence: 98%

“…Cell lines expressing a high level of receptor were selected by FACS and were cloned by limiting dilution. The ELISA employed anti-(insulin receptor) monoclonal antibody (mAb) 83.7 as the capture antibody and biotin-labelled mAb 83.14 for detection [39]. In FACS analysis, cells were treated with mAb 83.7 followed by FITC-labelled antimouse secondary antibody from sheep.…”

Section: Transfection and Screeningmentioning

confidence: 99%

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Mutational analysis of the N-linked glycosylation sites of the human insulin receptor

Elleman

Frenkel

Hoyne

et al. 2000

Biochemical Journal

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Site-directed mutagenesis has been used to remove 15 of the 18 potential N-linked glycosylation sites, in 16 combinations, from the human exon 11-minus receptor isoform. The three glycosylation sites not mutated were asparagine residues 25, 397 and 894, which are known to be important in receptor biosynthesis or function. The effects of these mutations on proreceptor processing into α and β subunits, cell-surface expression, insulin binding and receptor autophosphorylation were assessed in Chinese hamster ovary cells. The double mutants 16j78, 16j111, 16j215, 16j255, 337j418, the triple mutants 295j337j418, 295j418j514, 337j418j514 and 730j 743j881 and the quadruple mutants 606j730j743j881 and 671j730j743j881 seemed normal by all criteria examined. The triple mutant 16j215j255 showed only low levels of correctly processed receptor on the cell surface, this processed receptor being autophosphorylated in response to insulin. The quadruple mutant 624j730j743j881 showed normal pro-

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Section: Whole Hir Mutantsmentioning

confidence: 98%

Section: Transfection and Screeningmentioning

confidence: 99%

Mutational analysis of the N-linked glycosylation sites of the human insulin receptor

Elleman

Frenkel

Hoyne

et al. 2000

Biochemical Journal

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“…The details of the injection volume and injection procedure were described previously (Murakami et al, 2013). This antibody blocks the binding between insulin and insulin receptors (Soos et al, 1986;Taylor et al, 1987). The control experiments were performed by injection of IgG (4.4 µg ml −1 as its final concentration in Lymnaea saline; whole molecule, Jackson ImmonoResearch Laboratories, West Grove, PA, USA; Murakami et al, 2013).…”

Section: Injection Of Insulin Receptor Antibodymentioning

confidence: 99%

Memory block: A consequence of conflict resolution

Ito

Yamagishi

Hatakeyama

et al. 2015

Journal of Experimental Biology

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Food deprivation for 1 day in the pond snail Lymnaea stagnalis before aversive classical conditioning results in optimal conditioned taste aversion (CTA) and long-term memory (LTM) formation, whereas 5-day food deprivation before training does not. We hypothesize that snails do in fact learn and form LTM when trained after prolonged food deprivation, but that severe food deprivation blocks their ability to express memory. We trained 5-day food-deprived snails under various conditions, and found that memory was indeed formed but is overpowered by severe food deprivation. Moreover, CTA-LTM was context dependent and was observed only when the snails were in a context similar to that in which the training occurred.

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“…The insulin receptor kinase was purified to apparent homogeneity using a 'single-step' immunoadsorption technique employing a monoclonal antibody raised against a pure human insulin receptor preparation. This has been described in detail elsewhere [22,23]. Purification of Gt and G, to apparent homogeneity was done as described in some detail by one of us [lo].…”

Section: Pre-incubation Mixturementioning

confidence: 99%

The insulin receptor tyrosyl kinase phosphorylates holomeric forms of the guanine nucleotide regulatory proteins G_i and G_o

et al. 1987

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An affinity purified human insulin receptor preparation was shown to phosphorylate the LY-and B-subunits of the guanine nucleotide-regulatory proteins Gi and G,, derived from bovine brain. The presence of insulin stimulated the rate of their phosphorylation some 2-fold. The presence of Gi and G, did not affect the degree of autophosphorylation of the B-subunit of the insulin receptor. Under conditions known to cause the dissociation of G, and G, into their constituent subunits then phosphorylation of Gi and G, by the insulin receptor was abolished. The cr-subunits of G, and G, could be selectively phosphorylated by the insulin receptor tyrosylkinase using appropriate concentrations of Mg2+ and GTP-y-S.

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Monoclonal antibodies reacting with multiple epitopes on the human insulin receptor

Cited by 195 publications

References 45 publications

Mutational analysis of the N-linked glycosylation sites of the human insulin receptor

Mutational analysis of the N-linked glycosylation sites of the human insulin receptor

Memory block: A consequence of conflict resolution

The insulin receptor tyrosyl kinase phosphorylates holomeric forms of the guanine nucleotide regulatory proteins G_i and G_o

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Monoclonal antibodies reacting with multiple epitopes on the human insulin receptor

Cited by 195 publications

References 45 publications

Mutational analysis of the N-linked glycosylation sites of the human insulin receptor

Mutational analysis of the N-linked glycosylation sites of the human insulin receptor

Memory block: A consequence of conflict resolution

The insulin receptor tyrosyl kinase phosphorylates holomeric forms of the guanine nucleotide regulatory proteins Gi and Go

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Product

Resources

About

The insulin receptor tyrosyl kinase phosphorylates holomeric forms of the guanine nucleotide regulatory proteins G_i and G_o