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(Received for publication, July 17, 1995; and in revised form, August 23,
1995) The cDNA encoding QPc-9.5 kDa (subunit VII) of bovine heart
mitochondrial ubiquinol-cytochrome c reductase was cloned and
sequenced. This cDNA is 665 base pairs long with an open reading frame
of 246 base pairs that encodes an 81-amino acid mature QPc-9.5 kDa. The
insert contains 395 base pairs of a 3`-noncoding sequence with a
poly(A) tail. The amino acid sequence of QPc-9.5 kDa deduced from this
nucleotide sequence is the same as that obtained by protein sequencing
except that residue 61 is tryptophan instead of cysteine. The QPc-9.5
kDa was overexpressed in Escherichia coli JM109 cells as a
glutathione S-transferase fusion protein (GST-QPc) using the
expression vector, pGEX/QPc. The yield of soluble active recombinant
GST-QPc fusion protein depends on the induction growth time,
temperature, and medium. Maximum yield of recombinant fusion protein
was obtained from cells harvested 3 h postinduction of growth at 27
°C on LB medium containing betaine and sorbitol. QPc-9.5 kDa was
released from the fusion protein by proteolytic cleavage with thrombin.
Isolated recombinant QPc-9.5 kDa showed one protein band in
SDS-polyacrylamide gel electrophroesis corresponding to subunit VII of
mitochondrial ubiquinol-cytochrome c reductase. Although the
isolated recombinant QPc-9.5 kDa is soluble in aqueous solution, it is
in a highly aggregated form, with an apparent molecular mass of over 1
million. Addition of detergent deaggreates the isolated protein to the
monomeric state, suggesting that the recombinant protein exists as a
hydrophobic aggregation in aqueous solution. The recombinant QPc-9.5
kDa binds ubiquinone and shows a spectral blue shift. Upon titration of
the recombinant protein with ubiquinone, a saturation behavior is
observed, suggesting that the binding is specific and that the
recombinant protein may be in the functionally active state.
Volume 270,
Number 43,
Issue of October 27, 1995 pp. 25634-25638
©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
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