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. 2017 Nov 27;67(2):265–277. doi: 10.2337/db17-0321

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© 2017 by the American Diabetes Association.

Readers may use this article as long as the work is properly cited, the use is educational and not for profit, and the work is not altered. More information is available at http://www.diabetesjournals.org/content/license.

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The Clec16a-Nrdp1-USP8 complex is perturbed by glucolipotoxicity. A: Top, representative deconvolution image of Nrdp1:USP8 Proximity Ligation Assay (PLA, red; DAPI, blue) in Min6 β-cells 72 h after transfection with nontargeting (NT) or Clec16a-specific shRNA plasmids after treatment with BSA control or 0.4 mmol/L palmitate for 48 h; bottom, quantification of relative Nrdp1:USP8 PLA events in Min6 β-cells (fold change vs. NT shRNA BSA controls). (n = 4/group and ∼1,200 PLA events quantified/group per experiment.) B: Top, representative deconvolution image of Nrdp1:USP8 PLA (PLA, red; PDX1, green; and DAPI, blue) in β-cells of dissociated human islets after 48 h treatment with BSA control (BSA) or 0.4 mmol/L palmitate and 0.92% BSA + 20 mmol/L glucose (palmitate); bottom, quantification of relative Nrdp1:USP8 PLA events in β-cells of dissociated human islets after control BSA (white bar) or 0.4 mmol/L palmitate and 0.92% BSA + 20 mmol/L glucose (gray bar) treatment for 48 h (n = 3 donors and ∼900 β-cell PLA events quantified/group per donor). C: Top, representative Western blot (WB) of Nrdp1 levels in isolated mouse islets treated for 48 h with or without 0.4 mmol/L palmitate + 20 mmol/L glucose; bottom, relative quantification (by densitometry) of Nrdp1 levels by Western blot in isolated islets from mice treated for 48 h with (gray bars) or without (white bars) 0.4 mmol/L palmitate and 0.92% BSA + 20 mmol/L glucose. n = 3/group. D: Representative Western blot of in vivo ubiquitination assay of HA-Nrdp1 in Min6 cells transfected with HA-Nrdp1, Myc-tagged ubiquitin (Myc-Ub), and Flag–empty vector or Flag-Clec16a plasmids and treated for 48 h with or without 0.4 mmol/L palmitate/BSA coupling. n = 3/group. E: Representative Western blot after Flag-immunoprecipitation (IP) in Min6 cells transfected with HA-Nrdp1, Flag-USP8, and either GFP–empty vector or GFP-Clec16a plasmids and treated for 48 h with or without 0.4 mmol/L palmitate. n = 4/group. F: Top, representative WB of cleaved caspase-3 levels in Min6 cells transfected with or without GFP-Clec16a and treated for 48 h with BSA or palmitate; bottom, relative quantification (by densitometry) of cleaved caspase-3 levels (normalized to actin loading control) by Western blot in Min6 cells transfected with or without GFP-Clec16a and treated for 48 h with BSA (white bars) or palmitate (gray bars) couplings. n = 5/group. *P < 0.05, ***P < 0.001, nonpaired Student t test. ns, not significant.