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Fig. 5. CUP interacts with TIC. (A) The interaction between CUP and TIC, first
detected in a yeast two-hybrid screen, was confirmed by GST pulldown. The
lanes labelled CUP and TIC contain in vitro synthesised, radiolabelled CUP and
TIC protein controls, respectively. The lanes labelled CUP* and
TIC* contain the pulldown products resulting from combining
labelled CUP or TIC with GST-fusion proteins with CUP (CUPG) or TIC
(TICG) or GST alone. The strong band in the
CUP*TICG lane corresponds to an interaction between
labelled CUP and GST-TIC. A weaker band in the TIC*CUPG
lane shows the interaction between labelled TIC and GST-CUP. A band is also
observed in the TIC*TICG lane, indicating that TIC also
interacts with itself. (B) The tissue specific expression of TIC and
CUP was investigated by RT-PCR (35 cycles) using RNA derived from
leaf (L), inflorescence (I), sepal (Se), petal (P), stamen (St) and carpel (C)
tissues. The expression pattern of CUP is as expected from in situ
hybridisation experiments, being absent from mature leaves, sepals and
stamens, and present in carpels and petals. The strongest expression is
detected in inflorescences, where in situ hybridisation shows that
CUP is expressed at the many boundaries between developing meristems
and primordia. The expression pattern of TIC broadly follows that of
CUP, but shows a wider tissue distribution. Equal loading is shown by
an elongation factor control.
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