Post-translational selective intracellular silencing of acetylated proteins with de novo selected intrabodies

(a) PISA technology combines chimeric tethered catalysis constructs and IACT method to select intrabodies against a desired acetylated protein target. The protein target is fused to the LexA DNA Binding Domain (LexA DBD), for the two hybrid selection, and to an acetylating enzyme (HAT), for acetylation of the protein target. Acetylation (Ac) of the native-folded protein target is catalyzed in cis, by the wild type HAT enzyme, directly in the yeast intracellular environment. The acetylated protein, fused to LexA DBD, which binds LexA promoter inserted in the yeast L40 genome. When a specific anti-acetylation scFv (from a scFv library) is co-transformed together with the acetylated protein target, yeast growth is permitted, due to the transcriptional activation of HIS3 gene, which is required for L40 strain survival. HIS3 transcription is allowed by VP16 Activation Domain, which is fused to the intracellular scFv. (b) Yeast cells expressing an intrabody (from the scFv library) which is not binding the acetylated protein bait do not grow, since intrabody/bait binding is required for yeast survival. (c) Specificity of the selected scFv anti-acetylation binders is ensured by a counter-screening. The anti-acetylation intrabody candidate (in green) is challenged with a control version of the bait, in which the HAT enzyme is mutated, and the protein target is therefore non-acetylated. In this case, no binding occurs, and no growth is observed. HAT= Histone Acetyl Transferase, DBD=DNA Binding Domain, AD= Activation Domain, ScFv=Single Chain Fragment Variable. The PISA screening, in principle, is not limited to scFv libraries, but functions with repertoires of different binding domains, such as Nanobodies, VH domains, DARPins, or others.

(a) Schematic representation of tethered catalysis baits for PISA screening. Target antigen is fused at the C-terminus of LexA DNA Binding Domain (DBD) and at the N-terminus of a Histone Acetyl Transferase (HAT) catalytic domain. As descried in Guo et al. (Nat. Biotechnol., 888–892 (2004)), the antigen is post-translationally modified in a constitutive manner by the wild type version of the enzyme (left, screening bait), but it is not modified when HAT is mutated with an inactivating single point mutation (right, control bait). (b) Histone H3 (H3) and Integrase (IN) baits were expressed in yeast and immunoprecipitated with anti-HA antibody (rat monoclonal). After IP, their expression was verified by Western Blot using anti-HA Ab (rabbit polyclonal). Acetylation has also been verified with either an anti-H3Ac antibody or an anti-acetyl-lysine antibody.

(a) LexA control baits used for epitope mapping are expressed in yeast to investigate their correct expression, as done for the screening baits. The only bait that does not carry a HA tag is LexA-Integrase, whose expression is shown, in the central figure, for two different clones (CFUs). (b) Auto-activation assay for screening and control baits. Yeast baits spotted on histidine-lacking plates in which 3-AT is titrated, allow identification of auto-activation level. The 3-AT concentration, at which non-specific growth (in the absence of an interactor) is arrested, is included in the medium when testing an intrabody interaction. H3 screening bait (LexA-H3-Gcn5wt-HA) needs at least 5mM 3AT, while other control baits are grown at 1.25mM 3AT. As for the Integrase bait panel, LexA-IN-P300wt-HA does not show any auto-activation, unlike LexA-P300wt-HA and LexA-IN which require 1.25mM 3AT.

(a) LexA-Integrase bait (IN(1) and (2) on the left are different clones) is expressed at comparable levels as LexA-IN-P300-HA baits on the right part of the panel (anti-Integrase western blot). (b) If the same samples are blotted for anti-acetyl-lysines, signal is detected only in the lane corresponding to the P300 wild type chimera (IN-P300wt-HA).

(a) Yeast growth on histidine-lacking plates (with the addition of appropriate 3AT concentration, a His3 inhibitor) demonstrates interaction specificities for 112A and 12X intrabodies. In particular, it is shown how the splitting of ScFvs in its constituent Variable domains abolishes its cross-reactivity with P300mut for both VH-112A and VH-12X. The panel a illustrates VH-112A to be a specific anti-acetyl-Integrase intrabody, and VH-12X to target Integrase regardless of its acetylation status. (b) Yeasts are restreaked from transformation plates on fresh selective plates. The effect of splitting ScFv-112A variable domains is consistently evident. (c) Beta-galactosidase lift assays performed on restreaked colonies carrying 112A/Integrase prey/bait pairs further confirm the specific acetyl-Integrase binding of VH-112A, compared to its ScFv version. (d) Cross-reaction between P300mut bait and anti-Integrase intrabodies (ScFv-112A and ScFv-12X) is totally suppressed by a low dose of 3AT (1.25mM), which is the same that was used to suppress transactivation of P300wt bait (see Supplementary Figure 3b). The panel shows three independent clones of ScFv-112A and ScFv-12X restreaked from the transformation plate.

His-Integrase recombinant protein is purified from E. coli and used as a substrate of P300 acetyl-transferase, in the presence of Ac-CoA. Acetylation occurs, in vitro, upon addition of either full-length P300 protein (second lane) or of its catalytic domain only (third lane), with no difference in yield. As a control, a commercial preparation of Histone Cores (lane 4 and 5) is tested with both enzyme variants. Last two lanes demonstrate how addition of mutated, recombinant version of P300 does not induce acetylation of the Integrase protein or Histones. WB in the bottom panel shows comparable levels of His-tagged Integrase in each preparation. Bands at >75kDa reflect auto-acetylation of P300 enzyme, as previously reported in literature. Anti-His WB is used to confirm the presence of the Integrase recombinant protein in its both acetylated and non-acetylated forms.

(a) Co-IP of VH-12X-HA with His-tagged acetyl integrase versus integrase, using anti-His (left) or anti-HA (right) blotting. (b) HIV infectivity assay. Cytoplasmic localization of the intrabody. Graph shows percentage of GFP+ cells after intrabody transfection and viral transduction. CTRL+ represents the non-transfected control. (c) HIV infectivity assay. Nuclear localization of the intrabody. Graph shows percentage of GFP+ cells after intrabody transfection and viral transduction. CTRL+ represents the non-transfected control. The Kolmogorov-Smirnov test was used to assess the normality of the samples. Then, F test for determining homoscedasticity between samples was applied, followed by appropriate t-test of means comparison. For each comparison, t-test corrections for heteroscedasticity (Welch's t-test) were used when needed. Each experiment was repeated at least twice. Infectivity data shown as whiskers and boxes plots. Boxes of graphs (b) and (c) represent distribution of first to third quartiles, while internal line represents the median. Whiskers represent min and max values. The intrabody transfection efficiency was in the range of 70 +/- 5 %.

Source data

(a) Liquid beta-galactosidase assay shows how ScFv-58F is the only intrabody that is able to recognize the screening bait exclusively. The right panel gives an idea of the interaction strength, which is proportional to color intensity. Values are normalized by subtraction of the negative control (ctrl- in the left figure) and reported as bar chart on the right. Y1 is an anti-LexA intrabody, used as the positive control (ctrl+). (b) Beta-galactosidase filter assay demonstrates the same interaction pattern observed with the liquid assay. Background levels of LacZ due to auto-activation are more evident in the filter assay than in the liquid assay (see the negative control of the H3-Gcn5wt panel).

(a) Co-IP between ScFv-58F-HA and purified His-H3/HisAcH3 proteins (both expressed in E.coli, H3 acetylated in vitro), using anti-HA agarose, followed by anti-HIS Western Blot. Lanes 1-2: bound fraction (quantification in Supplementary Figure 12). Lanes 3-4: unbound fraction. Lanes 6-7: anti-HA agarose immunoprecipitation in the absence of ScFv-58F. Lane 8: loading from the same His-H3 preparation. Inputs and acetylation status are shown on the right. Samples are analyzed with an anti-His-HRP antibody, which cross-reacted with ScFv-58F-HA. (b) Relative quantification by Western Blot of Acetylated Histone H3 in yeast expressing ScFv-58F, ScFv-112A or no intrabody (L40). Acetylated H3 band density from two biological replicates was normalized on Total H3. Data are shown as individual points and mean +/- S.D. N=2.

Source data

Data analysis performed with ActiveMotif software for the Histone MODified Annotated Array. ScFv-58F is strongly specificity for the acetylated lysine #9 of Histone H3 over other common modifications. Array is showed in Figure 2a.

(a) Direct ELISA performed with purified ScFv-58F against a panel of H3 histone peptides coated on solid phase. ELISA shows the specificity of ScFv-58F for H3K9Ac. Minor reactivity is observed towards the non-modified N-terminal peptide. (b) ELISA dilution binding curve using 10 μM of acetylated (K9) or non acetylated H3 peptides coated on solid phase and different concentrations of ScFv-58F-HA as probe. (c) ELISA dilution binding curve using native acetylated H3 protein and H3AcK9 peptide, both coated on solid phase. The curves show a concentration range where ScFv-58F binds more effectively to the native acetylated protein than to the acetylated peptide.

Relative quantification of Western Blot bands obtained in the pull-down assay shown in Supplementary Figure 9a. ImageJ software was used to perform densitometric analysis. Ac= Acetylated; n.a.= non acetylated.

(a, b) Membranes from which right panels of Supplementary Figure 9a are derived, showing inputs of in vitro acetylated/non-acetylated recombinant H3 Histone. In (b), anti-His PENTA by Qiagen cross-reacts with BioRad Dual Color marker (cross-reaction seen also in other blots at the dilution of 1:1000 – 1:2000 and for longer exposures). (c) Blot membrane from which Figure 2c is derived. First lane= BioRad Dual Color. From the fifth lane, samples are not relevant to the experiment, and were used as internal controls. (d) Membrane from which Figure 2c is derived. Last lane is another yeast extract used as internal control. (e, f) Western blot membranes of experiments shown in Supplementary Figure 9b. Lanes 5-7 are non-relevant for the experiment. For all gels, BioRad Dual Color marker was used.