Figure 4
Figure 4. ONOO− is downstream of O2− in the inhibition of PP2AB56δ holoenzyme assembly. (A) Intracellular NO was measured in DDC-treated Jurkat cells using a NO-sensitive probe, DAF-FM. (B) Jurkat cells were pretreated with FeTPPS for 1 hour, followed by DDC treatment, and then IB for the indicated proteins. (C) S70pBcl-2 status was assessed in Jurkat cells after a 2-hour treatment with the indicated concentrations of ONOO−. (D) Jurkat cells were treated with 10 μM ONOO− for 2 hours and harvested for co-IP assay with Bcl-2 as bait. (E) IB analysis of mitochondrial fractions from Jurkat cells preincubated with 100 μM FeTPPS followed by DDC or ONOO− treatment. (F) Multiple sequence alignment of B56 regulatory subunits of both mammalian and nonmammalian origin. The nitration-prone tyrosine residue (Y) identified in B56 family members is boxed in red. Blue arrows denote residues that are implicated in the interaction of B56 subunits with PP2A-A.28 Adjacent residues proposed to predispose a tyrosine residue toward nitrative modification process are indicated by red, green, and purple arrows (refer to supplemental Figure 5C for details). Multisequence alignment analysis was performed via Jalview 2.7. (G-H) Lysates from DDC (with or without FeTPPS pretreatment) and ONOO−-treated Jurkat cells were IP using anti-B56δ Ab and IB for 3-NT and other indicated proteins. (I) Twenty-four hours after SOD1 silencing, Jurkat cells were treated with 2.5 μM DPI for an additional 24 hours and harvested for co-IP analysis using the indicated Abs. (J) Lysates from bSOD1 treated (16 hours, 1 kU) or SOD1-overexpressing Jurkat cells were IP using anti-B56δ Ab and IB for 3-NT and other indicated proteins.

ONOO is downstream of O2 in the inhibition of PP2AB56δ holoenzyme assembly. (A) Intracellular NO was measured in DDC-treated Jurkat cells using a NO-sensitive probe, DAF-FM. (B) Jurkat cells were pretreated with FeTPPS for 1 hour, followed by DDC treatment, and then IB for the indicated proteins. (C) S70pBcl-2 status was assessed in Jurkat cells after a 2-hour treatment with the indicated concentrations of ONOO. (D) Jurkat cells were treated with 10 μM ONOO for 2 hours and harvested for co-IP assay with Bcl-2 as bait. (E) IB analysis of mitochondrial fractions from Jurkat cells preincubated with 100 μM FeTPPS followed by DDC or ONOO treatment. (F) Multiple sequence alignment of B56 regulatory subunits of both mammalian and nonmammalian origin. The nitration-prone tyrosine residue (Y) identified in B56 family members is boxed in red. Blue arrows denote residues that are implicated in the interaction of B56 subunits with PP2A-A.28  Adjacent residues proposed to predispose a tyrosine residue toward nitrative modification process are indicated by red, green, and purple arrows (refer to supplemental Figure 5C for details). Multisequence alignment analysis was performed via Jalview 2.7. (G-H) Lysates from DDC (with or without FeTPPS pretreatment) and ONOO-treated Jurkat cells were IP using anti-B56δ Ab and IB for 3-NT and other indicated proteins. (I) Twenty-four hours after SOD1 silencing, Jurkat cells were treated with 2.5 μM DPI for an additional 24 hours and harvested for co-IP analysis using the indicated Abs. (J) Lysates from bSOD1 treated (16 hours, 1 kU) or SOD1-overexpressing Jurkat cells were IP using anti-B56δ Ab and IB for 3-NT and other indicated proteins.

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