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Fig. 6. NHR-25 binds to the wild-type, but not the e1417, form of ACEL.
(A) A cis-element in the ACEL, which contains the e1417 mutation
site, is similar to the FTZ-F1 binding site consensus. (B) Two forms (
-
and ß-) of nhr-25 cDNA. DB represents a DNA binding domain and
LB a ligand-binding domain. Both messages are trans-spliced with SL1 RNA. The
-form contains an intact DNA-binding domain and the ß-form
partially deletes the domain. (C) Synthesis of both forms of the NHR-25
protein. The proteins were synthesized using in vitro transcription and
translation (TNT) in rabbit reticulocyte lysates with
35S-methionine. The proteins were visualized by autoradiography
after SDS-PAGE. (D) EMSA showing the binding of NHR-25 to the wild-type ACEL
DNA probe. The - and ß- NHR-25 proteins, which were synthesized
using in vitro TNT with cold methionine, were incubated with the
32P-labeled wild-type (wt) or e1417 form of ACEL DNA
probes. The reaction mixtures were separated on a non-denaturing
polyacrylamide gel and the radioactivity signals were detected by
phosphoimager. F indicates the migration of free DNA probes, NS indicates the
migration of a non-specific protein/DNA probe complex, and B is the NHR-25/DNA
probe complex. An equal amount of non-specific protein/DNA probe complex (NS)
was observed in all of the binding reactions, regardless of the synthesis of
NHR-25, showing that equal amounts of the reticulocyte lysates were used for
the binding assay.
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