Further characterization of the Chi-dependent protease cleavage of RecC. (a)
RecBCD enzyme was reacted with uncapped lambda Chi0 or Chi+ DNA, as
in Fig. 2, or with lambda substrates capped at the
left or right end of lambda, marked L and R, to block RecBCD entry at the capped end. Chi
is active only if RecBCD enzyme enters from the right end [8]. Reactions were with 5 mM ATP and 2.5 mM Mg2+ (low
Mg2+) or 8 mM Mg2+ (high Mg2+), as shown, and reacted
with 10 nM trypsin for 1 min before Western blot analysis using RecC-specific polyclonal
antibodies. (b) As in (a) but showing polypeptides detected with anti-RecB polyclonal
antibodies. (c) Quantification of the Chi-dependent fragment in (a) and in parallel
reactions that used 3.2 and 32 nM trypsin; x and o, Chi+ and Chi0
reactions; L and R, left- and right-end caps. (d) Persistence of RecC’s
Chi-dependent sensitization to trypsin. RecBCD was reacted with Chi+ or
Chi0 DNA for 1 min; the reactions were stopped by addition of EDTA to 23 mM,
incubated for the further times indicated, and then treated for 1 min with 160 nM trypsin.
RecC fragments were detected as in Fig. 2. Continuous
and broken lines, ~91-kDa Chi-dependent fragment 1 and ~82-kDa
Chi-independent fragment 2. (e) DNA substrate used in (a), (b), and (c). Phage lambda DNA
(48.5 kb) with a Chi site (χ+D) 3.5 kb from the right
end. Hairpin DNA (gray, data not drawn to scale) ligated in some cases to one strand at
one or the other end of the lambda DNA substrate prevents RecBCD from unwinding from the
capped end. Arrow, direction RecBCD must unwind DNA to be changed by
χ+D [8].