PKL Interacts with BZR1.
(A) In vitro pull-down assay between recombinant His-BZR1 and
various PKL fragments tagged with GST. His-BZR1 proteins were incubated with
immobilized GST or GST-PKL, and immunoprecipitated fractions were probed with
an anti-His antibody. IB, immunoblot; IP, immunoprecipitation.
(B) Yeast two-hybrid assay between BZR1 fused with the B42
activation domain (AD) and the D2, D3, or D6 fragment of PKL (Supplemental Figure 1A) fused with the LexA DNA binding
domain.
(C)
BiFC assay showing that
YFPN-PKL and BZR1-YFPC interact to form a functional YFP
in the nucleus of Arabidopsis protoplasts. Chlorophyll,
chlorophyll autofluorescence; YFP, YFP fluorescence; merged, chlorophyll and
YFP fluorescence. Bar = 5 μm.
(D) Effect of BR
biosynthesis inhibition on seedling growth. The panels show phenotypes of Col wild-type, epp1,
pif3, and epp1 pif3 seedlings grown in
medium with or without 1 μM of the BR biosynthesis inhibitor PCZ in darkness for 5 d. Bars = 2 mm.
(E) Relative hypocotyl lengths of seedlings grown in various
concentrations of PCZ for 5 d. Data
represent means ± sd of at least 20 seedlings.
(F)
ChIP-qPCR assay showing the relative
enrichment of IAA19, PRE1, and
ACT2 (negative control) genomic fragments upon
precipitation with an anti-PKL antibody. Col and bzr1-1D seedlings were grown in darkness
for 5 d. Data represent means ± sd of three biological
replicates. Asterisks indicate significant differences from the wild type at P
< 0.05 (*) or P < 0.01 (**) using Student’s
t test.
(G) Immunoblot assay for PKL in the bzr1-1D
mutant. Immunoblotting against tubulin antibody served as the loading
control.