From the Departments of Biology, Human Genetics, and Pediatrics, McGill University Health Center-Montreal Children's Hospital Research Institute, Montréal, Québec H3Z 2Z3, Canada
Received for publication, October 24, 2000, and in revised form, December 15, 2000
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ABSTRACT |
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Biotin functions as a covalently bound cofactor
of biotindependent carboxylases. Biotin attachment is catalyzed
by biotin protein ligases, called holocarboxylase synthetase in mammals and BirA in prokaryotes. These enzymes show a high degree of
sequence similarity in their biotinylation domains but differ markedly in the length and sequence of their N terminus. BirA is also the repressor of the biotin operon, and its DNA attachment site is located
in its N terminus. The function of the eukaryotic N terminus is
unknown. Holocarboxylase synthetase with N- and C-terminal deletions
were evaluated for the ability to catalyze biotinylation after
expression in Escherichia coli using bacterial and human acceptor substrates. We showed that the minimum functional protein is
comprised of the last 349 of the 726-residue protein, which includes
the biotinylation domain. Significantly, enzyme containing intermediate
length, N-terminal deletions interfered with biotin transfer and
interaction with different peptide acceptor substrates. We propose that
the N terminus of holocarboxylase synthetase contributes to
biotinylation through N- and C-terminal interactions and may affect
acceptor substrate recognition. Our findings provide a rationale for
the biotin responsiveness of patients with point mutations in the
N-terminal sequence of holocarboxylase synthetase. Such mutant
enzyme may respond to biotin-mediated stabilization of the
substrate-bound complex.
Biotin is a water-soluble molecule essential for all forms of
life. From bacteria to animals and plants, biotin is used as a cofactor
in various carboxylation and decarboxylation reactions (reviewed in
Refs. 1-3). In Escherichia coli, a single enzyme, acetyl-CoA carboxylase, requires biotin as a cofactor. However in
mammals, four enzymes, acetyl-CoA carboxylase, methylcrotonyl-CoA carboxylase, propionyl-CoA carboxylase, and pyruvate carboxylase, utilize biotin. In such species, biotin is covalently linked to the
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-amino group of a lysine residue, which is part of the conserved (A/V)MKM sequence (3). The attachment of biotin to the lysine residue
is enzymatically catalyzed by biotin protein ligase
(BPL).1 In E. coli, BirA adds biotin to the biotin carboxyl carrier protein (BCCP) of acetyl-CoA carboxylase, whereas in mammals, plants, and
yeast, holocarboxylase synthetase (HCS) adds biotin to the respective
domain of each biotin-dependent enzyme. The BPL attaches the biotin to the apocarboxylase in an ATP-dependent
process that occurs in the following two half-reactions.
To attach biotin to its substrate, the BPL recognizes a
60-90-amino acid domain containing the acceptor lysine residue (3). The biotin binding site is often part of a larger subunit of the carboxylase enzyme. E. coli BCCP is a 156-amino acid
polypeptide of which only the last 82 are required for biotin
attachment by the BirA protein (4, 5). The 1.3 S biotin acceptor
subunit of Propionibacterium shermanii transcarboxylase is a
123-amino acid peptide of which the last 75 have been shown to be
sufficient to be biotinylated (6). Human pyruvate carboxylase, a
homotetramer of a 1180-amino acid polypeptide, has its biotin acceptor
sequence confined to the last 86 residues of the protein (referred to
as p-86, Ref. 7). Human propionyl-CoA carboxylase, a heteropolymer of
- and
-subunits, contains its biotin binding region in the last
67 of the 703-amino acid
-subunit (referred to as p-67, Ref. 8). All
of these sequences have been expressed independently of their larger
polypeptide and are readily biotinylated in vitro. BCCP and
the 1.3 S subunit have been characterized structurally and have been
shown to share a similar three-dimensional structure, which is related
to the lipoic acid binding domains of dehydrogenase multienzyme
complexes (9-12).
BPLs share a common catalytic domain (see Fig. 1), which was initially determined from the crystal structure of E. coli BirA complexed with biocytin (biotinyl-lysine, Ref. 13). It spans about 130 of the 321 amino acids of BirA. This sequence also shows a high level of identity with sequences in the C-terminal half of the human, yeast, and Arabidopsis enzymes (3). In E. coli BirA, the N terminus contains a DNA binding domain involved in transcription repression of the biotin operon (14-16). In contrast, the N terminus of the 726-amino acid human HCS is unrelated to the bacterial sequence and has no known role in transcriptional regulation (17). The yeast BPL shares some resemblance to the human enzyme, encoding a polypeptide of 690 amino acids (18, 19). A cDNA for the Arabidopsis thaliana BPL has recently been cloned and found to encode a protein of 367 amino acids (20, 21). This BPL is similar to the bacterial enzyme except for a chloroplast-targeting sequence at its N terminus.
Years ago, it was shown that BPLs were interchangeable between organisms (6, 22-25). More recently, this has been applied to the expressed biotin attachment domains as substrates, where E. coli BirA has been shown to successfully biotinylate BCCP87 (E. coli), p-75 (P. shermanii), p-86 (yeast), and p-67 (human) among the above carboxylases (6-8, 26). This made it possible to clone BPLs by functional complementation between species, and this has been accomplished for the human, Bacillus subtilis, A. thaliana, and yeast BPLs using a temperature sensitive E. coli BirA mutant as host (17-20).
Cloning of human HCS allowed the first functional dissection of an
eukaryotic BPL through mutation analysis of patients suffering from an
inherited deficiency of HCS activity. This deficiency results in
depressed activity of all four biotin-dependent
carboxylases, hence the term early onset "multiple carboxylase
deficiency" to describe the disease (27-30). Most patients with HCS
deficiency can be successfully treated with pharmacologic doses of
biotin (27, 31, 32), and several point mutations have been localized to
the region of homology between BirA and HCS (see Fig. 1; Refs. 33, 34).
HCS containing these mutations has been shown to be "biotin
responsive" in expression experiments and has been shown to be
defective in biotin binding (35-37). Several other point mutations
(R183P, L216R, L237P, V333E, and V363D) form a cluster outside the
region of homology and, as such, appear to define a distinct region
important for HCS activity (35-39). This suggests that some residues
in the N-terminal domain of HCS might participate in the reaction even
though this region has no bacterial counterpart. To test this
hypothesis, we randomly generated N-terminal deletions and tested their
effect on HCS activity toward either the human (p-67) or bacterial
peptide substrates (BCCP or BCCP-87). Also, two C-terminal deletions
were engineered to test the importance of the C-terminal domain.
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EXPERIMENTAL PROCEDURES |
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Materials and Reagents-- E. coli strain birA104 and purified apoBCCP87 were the kind gifts of A. Campbell (Stanford University) and D. Beckett (University of Maryland at College Park), respectively. p-67 was expressed and purified using the Pichia pastoris expression system from Invitrogen.2 The exo-size deletion kit was from New England BioLabs, [14C]biotin (53 mCi/mmol) from Dupont Chemicals, IPTG from Life Technologies, Inc., the Wizard miniprep kit from Promega, and the Qiafilter Midiprep kit from Qiagen. The High Fidelity long PCR kit was from Roche Molecular Biochemicals. Mouse MGRS-His antibody and Ni2+-NTA-agarose were from Qiagen. All subcloning and plasmid transfections for vector constructions were done in E. coli TOP10F'.
Subcloning of HCS into the Expression Vector-- We used the shortest functional HCS clone (clone BL-04) that we previously isolated by functional complementation of birA104 (17). It encodes a protein of 669 amino acids counting from Met-58 relative to the full-length 726-amino acid enzyme. Both isoforms have previously been shown to have equivalent activity (Ref. 17).3 This cDNA was subcloned from the original pSE936 plasmid (40) into the EcoRI site of Bluescript SK-. The plasmid was digested with SmaI and HindIII for subcloning the cDNA into the pQE30 poly(His) expression vector (Qiagen) to generate pQE30/HCS04. HCS expression could then be induced with IPTG, and the protein produced was fused with a polyhistidine tag (MRGS-His6) at its N terminus.
Generation of N-terminal Deletions of HCS-- The exo-size deletion kit was used following the manufacturer's instructions to generate unidirectional-nested digestion of double-stranded DNA. The pQE30/HCS04 plasmid was digested with SmaI and SacI, treated with mung bean nuclease for various times, religated, and transfected into E. coli TOP10F'. Colonies were picked and analyzed by sequencing and restriction endonuclease digestion. When required, the reading frame was restored by excising the corresponding insert with SphI and HindIII and placing it into the pQE31 or pQE32 version of pQE30. Other deletions were made using restriction endonuclease sites present in the cDNA. In one, the HCS cDNA in Bluescript was digested with KpnI/HindIII and inserted in the pQE32 to generate an HCS starting at R290. In another, digestion with PstI/HindIII and insertion in pQE31 generated an HCS starting at L460. Boundaries were verified by sequencing to confirm the reading frame and conservation of restriction sites.
Generation of C-terminal Deletions of HCS-- We used long PCR with oligonucleotides encoding restriction endonuclease sites to generate C-terminal deletions of HCS. HCS ending at L695 was generated from the HCS cDNA in Bluescript using the following oligonucleotides (written 5' to 3') for the long PCR: CTCGAGCTCCACGAAGGCCGGACG (primer I) and GGTGACCCGGGAGGAAGCCAGAAT (restriction sites used for subcloning underlined). The PCR product was digested with SacI/SmaI and inserted into pQE32. For HCS ending at G655, the primers were: primer I and GGAAGGAAGCTTGTTGGGCCCTTT. The PCR product was digested with SacI/HindIII and inserted into pQE32. As a control, the complete HCS cDNA (clone BL-04) was also amplified by long PCR, subcloned into pQE32, and tested for its ability to complement birA104. It was amplified with primer I and GACGCCCGGGATTACCGCCGTTT. The PCR product was digested with SacI/SmaI for subcloning. Each construct was generated twice from two independent PCR reactions. Plasmid constructs were verified by sequencing the insert boundaries. The various constructs were purified using the Qiafilter Midiprep kit, and 50-100 ng of plasmid were used to transfect competent E. coli birA104 that had already been transfected with plasmid pREP4 (Qiagen), encoding the lacIq repressor. Three colonies were picked for each construct and tested independently for reproducibility of results.
Measurement of HCS Activity by Complementation of birA104-- E. coli birA104 carrying each construct was streaked onto LB-agar plates containing 50 nM biotin, 2 mM IPTG, and 100 µg/ml ampicillin for incubation at the restrictive temperature of 42 °C or on plates containing 5 µM biotin, 2 mM IPTG, and 100 µg/ml ampicillin for incubation at the permissive temperature of 30 °C. In these conditions, growth of E. coli at 42 °C is directly correlated with the level of residual HCS activity.
Measurement of HCS Activity in Vitro--
Each construct was
tested for its ability to biotinylate the bacterial substrate BCCP or
the human substrate fragment, p-67 (8). The E. coli extract
was the source of unbiotinylated BCCP. E. coli birA104
harboring each construct was grown overnight at 30 °C in LB medium
containing 5 µM biotin and 100 µg/ml ampicillin. They
were diluted 1:100 in fresh LB with 5 µM biotin and 100 µg/ml ampicillin and grown at 30 °C until they reached an
A600 of 0.4-0.5. HCS expression was induced by
adding 2 mM IPTG and incubating the cells at 30 °C for
2 h. The cells were centrifuged and washed twice with
phosphate-buffered saline. They were resuspended in resuspension buffer
(50 mM potassium phosphate, pH 6.0, 1 mM
dithiothreitol, 10% glycerol, 1 mM phenylmethylsulfonyl
fluoride) and lysed by freeze-thaw in a methanol-dry ice water bath
followed by sonication. Protein concentrations were determined using
the Bio-Rad assay kit. For the HCS assay, 150 µg of protein lysate
was mixed with 25 µl of 2× biotinylation assay buffer (100 mM reduced glutathione, 600 mM Tris-HCl. pH
7.5, 50 mM MgCl2), 2 µl of 100 mM
ATP, 2 µl of [14C]biotin (0.1 µCi), and 5 µM p-67 in a final volume of 50 µl. Lysates were
incubated in duplicate at 42 °C for 1-2 h. After termination of the
reaction by the addition of 50 µl of SDS sample buffer (62.5 mM Tris-HCl, pH 6.8, 10% glycerol, 0.71 M
-mercaptoethanol, 3% SDS, 0.01% bromphenol blue), the lysates were
denatured 5 min at 100 °C and loaded onto a 12.5%
SDS-polyacrylamide gel and migrated at 30 mA for 3 h. Proteins
were transferred onto a nitrocellulose membrane by Western blotting
overnight at 34 V. The membranes were exposed to a Fujix-BAS 2000 Bioimaging analyzer phosphorimage plate to quantify the amount of
[14C]biotin incorporated into p-67 and/or BCCP. The
membranes were subsequently incubated with the MRGS-His antibody
according to the supplier's instructions for detection of the
poly(His)·HCS fusion protein.
Biotinylation of BCCP87 and p-67 by Purified HCS
Constructs--
Enzyme from several of the HCS constructs that showed
activity in the in vitro assay were purified on
Ni2+-NTA-agarose using the supplier's protocol.
Quantification of the partially purified HCS was done by
electrophoresis on a 12.5% SDS-polyacrylamide gel electrophoresis with
known amounts of purified BirA (kindly provided by D. Beckett) and
interpolating the concentration of HCS while correcting for the protein
size difference. Each HCS construct was tested for its ability to
biotinylate p-67, BCCP87, or p-67 and BCCP87 together. The final volume
of the reaction was 25 µl and contained 10 µM p-67 or
BCCP87 or a 5 µM mixture of each substrate, 1 µl of
[14C]biotin (0.05 µCi), 1 µl of 100 mM
ATP, 12.5 µl of 2× biotinylation assay buffer, and 0.5 µM of purified HCS. The samples were incubated for 1 h at 37 °C, and the reaction was stopped by addition of 25 µl of
SDS sample buffer. Samples were denatured and loaded on a 16% (49.5%
T, 6% C) 0.7 mm Tris/Tricine SDS-polyacrylamide gel (41) and migrated
at 35 mA for 6 h. Transfer onto nitrocellulose, exposure to the
phosphorimage plate, and detection of the BCCP87 and p-67 reaction
products and poly(His) fusion protein were done as in the in
vitro assay.
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RESULTS |
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Functional Analysis of poly(His)·HCS-- HCS clone BL-04, starting at Met-58 relative to the longest cDNA clone isolated by Leon Del Rio et al. (17), was subcloned into the E. coli expression vector pQE30 to generate pQE30/HCS4 as described under "Experimental Procedures." The HCS protein produced by this system is fused at its N terminus with a polyhistidine tag. This poly(His) HCS construct was tested for its ability to complement the temperature-sensitive E. coli mutant birA104. Transformation of birA104 with pQE30/HCS04 and incubation at the restrictive temperature of 42 °C results in normal growth comparable with that obtained for HCS fused to the lacZ gene in Bluescript or HCS expressed from plasmid pSE936 used in previous experiments (Ref. 35 and results not shown). No growth is obtained for birA104 grown alone at 42 °C. Western transfer of bacterial cell lysates onto nitrocellulose membranes and detection of the poly(His) fusion proteins using the MRGS-His antibody gives a protein of the expected size (see Figs. 2-5, Control or M58 lanes).
Effects of C-terminal Deletions on HCS Activity--
We designed
oligonucleotides encoding restriction endonuclease sites to subclone
C-terminal truncated versions of HCS after amplification by long PCR.
Two C-terminal deletions of HCS were generated: a 31-amino acid
deletion ending at Leu-695 and a 71-amino acid deletion ending at
Gly-655 (Fig. 1). Each deletion was
tested for its ability to complement E. coli birA104 at the
restrictive temperature of 42 °C, as well as for its ability to
biotinylate BCCP and p-67 in extract assays. Both C-terminal deletions
fail to complement birA104 at 42 °C and do not display
any biotinylating activity toward p-67 or BCCP in vitro
despite production of a protein of the expected size by Western blot
(Fig. 2). In contrast, full-length HCS
clones (from Met-58) generated similarly by long PCR support growth of
birA104 at 42 °C, show biotinylation of both substrates
in vitro and produce a protein of the expected size (Fig.
2).
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Ability of N-terminal-deleted HCS Constructs to Complement
birA104--
N-terminal deletions were generated by exonuclease
treatment and subcloned into reading frame variants of the expression
vector so as to permit expression of the truncated HCS. In this manner, eight N-terminal deletions were obtained with HCS starting at Ala-80, Leu-165, Leu-166, Ala-235, Thr-266, Pro-338, Lys-378, and Pro-569 (Fig. 1). Two additional constructs, generating HCS starting at Arg-290 and Leu-460, took advantage of restriction endonuclease sites present in the HCS cDNA. Each construct was tested for its ability to complement E. coli birA104 at the
restrictive temperature (Fig.
3A). HCS cDNAs starting at
Ala-80, Leu-165, or Leu-166 complement birA104 at 42 °C,
showing growth at levels only slightly less than obtained for Met-58.
In contrast, HCS starting at Ala-235 fails completely to complement the
E. coli mutant, providing an initial border to the minimum
functional enzyme. However, further deletion to Thr-266 shows partial
growth and still further deletion of N-terminal sequences to Arg-290, Pro-338 or Lys-378 restores growth to levels obtained for constructs starting at Met-58 to Leu-166. Finally, removal of additional sequences
to Leu-460 or Pro-569 completely abolishes growth of birA104. These data indicate that the complementing deletion
constructs generate truncated enzymes capable of biotinylating BCCP at
a level sufficient to support growth of the E. coli
mutant.
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In Vitro Assay of N-terminal-deleted Constructs-- Each of the N-terminal-deleted constructs was assayed in extracts for biotinylation of BCCP and p-67, the former derived from the broken cell extract and the latter added directly into the assay (Fig. 3B). Most of the in vitro assay results are in accord with those obtained by the complementation growth of birA104. Several HCS constructs that are able to complement birA104 (HCS starting at Met-58, Arg-290, Pro-338, and Lys-378) are able to biotinylate BCCP in vitro, whereas constructs unable to complement birA104 (HCS starting at Ala-235, Leu-460, Pro-569) fail to show BCCP biotinylation. One construct, HCS starting at Thr-266, which complements birA104 weakly, also shows weak biotinylation of BCCP. Some constructs are discordant between the complementation growth tests and the in vitro assays: HCS starting at Ala-80 is able to complement birA104 but does not incorporate any labeled biotin into BCCP in the in vitro assay. However, this proved to be because the BCCP was already fully biotinylated in culture, thereby preventing any further biotinylation in the extract assay. When the same log phase cell extract was mixed with an equivalent amount of a culture producing HCS starting at Ala-235 (negative by complementation and in vitro assay) to provide an independent source of unbiotinylated BCCP, transfer of biotin to BCCP was observed (result not shown). Western detection of the fusion protein also shows that the Ala-80 clone produced a higher level of HCS than the Met-58 control construct (Fig. 3C). Another discrepancy is with HCS starting at Leu-165 or Leu-166. Both constructs could complement birA104 but they do not show any activity in the in vitro assay or presence of the fusion protein by Western blotting. Production of an active but unstable protein that was rapidly degraded on cell lysis is the most likely explanation. Other discrepancies were noted in the competition between BCCP and p-67 as substrate for biotinylation. HCS starting at Met-58 biotinylates both BCCP and p-67 (Fig. 3B), whereas HCS starting at Arg-290 or Pro-338 shows biotinylation of BCCP, but no trace of labeled p-67 is detected. The ability to biotinylate both substrates is regained when HCS starts at Lys-378.
Comparison of BCCP87 and p-67 as Substrates for Purified
N-terminal-deleted Constructs--
The HCS from constructs giving a
stable protein and activity in the in vitro assay were
purified using Ni2+-NTA agarose to further examine their
substrate specificity. These included HCS starting at Met-58, Ala-80,
Arg-290, Pro-338, and Lys-378 (Fig. 4).
This procedure clearly shows enrichment of the derivative HCS by
Coomassie staining and Western blot, although the presence of
contaminating proteins or proteolytic products prevented direct
quantification of the isolated enzymes. Each sample was tested for
biotinylation of p-67, BCCP87, or an equimolar mixture of both
substrates (Figs. 1, 5). HCS starting at Met-58 and Ala-80 show
biotinylation of both BCCP87 and p-67 with a similar level of
biotinylation of the mixture. HCS starting at Arg-290 and Pro-338 fail
to biotinylate BCCP87 but show weak biotinylation of p-67, whereas HCS
starting at Lys-378 shows a much stronger biotinylation of p-67 and
weak biotinylation of BCCP87. These results for the purified Arg-290
and Pro-338 protein contrast with those obtained with the crude cell
lysates in which biotinylation of full-length BCCP was favored over
p-67. The BirA enzyme from a host expressing the wild-type sequence was
tested for its ability to biotinylate each substrate in this assay and,
as shown in Fig. 5 (top), both
BCCP87 and p-67 are biotinylated at similar levels. Detection of the
HCS fusion proteins by Western blotting shows that similar amounts of
enzyme were added in each set of assays (Fig. 5,
bottom).
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DISCUSSION |
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In this study, we showed that deletion of the first 377 amino acids of the 726 amino acid human HCS yields a protein that retains biotinylating activity, both in vivo and in vitro. This 349-amino acid segment contains the biotinylation domain, residues Gly-466 to Val-674 (3), that is homologous in all BPLs. This region contains the sites shown to make contact with biotin in the co-crystallized E. coli BirA-biocytin (biotinyl-lysine) complex (13). As well, it includes a sequence, G(K/R)GRXG, initially thought to be an ATP binding site in BirA but shown recently to be involved in biotin/biotin-AMP binding (42). It also includes a short segment (P/D)DGN(S/T)FD (residues 709-715) that is also found in yeast, A. thaliana, and Caenorhabditis elegans BPL, which may explain our finding of an absolute requirement for the C terminus by the human enzyme.
This initial result did not suggest a requirement for the N-terminal domain of HCS. However, intermediate deletions, leaving about two-thirds of the protein intact, interfered with biotinylating activity, suggesting that some level of interaction occurs between these two halves of the protein. In sum, a short deletion of 79 amino acids (that is, starting at Ala-80) resulted in a fully active enzyme. Additional deletions to generate proteins beginning at Leu-165 or Leu-166 also complemented the biotin auxotrophy of birA104 in vivo although they did not show any activity in vitro. These proteins were Western blot-negative, suggesting that the protein was unstable and rapidly degraded in cell homogenates. Significantly, further deletions to Ala-235 or Thr-266 were inactive or only partially active in vivo and in vitro, whereas removing still more residues to Arg-290, Pro-338, or Lys-378, restored biotinylating activity. Deletions to Leu-460 or Pro-569, which are within the biotinylation domain, were without any activity. These latter proteins, from Ala-235 onward except Pro-569, were all Western blot-positive indicating that stable proteins are generated from these constructs. We conclude that, in addition to the 349-amino acid active site domain, additional sequences, delimited by residues Leu-166 to Arg-290, interact with the biotinylation domain. Disruption of this N-terminal domain interferes with the biotin transfer reaction. We speculate that partial removal of Leu-166-Arg-290 inappropriately blocks the active site, whereas removing the domain altogether restores basal activity. Consistent with these findings, Narisawa and co-workers (37) reported recently that a truncated HCS initiating at Met-234 was inactive when expressed in human fibroblasts, whereas proteins initiating at Met-1, Met-58, and Ile-117 (with Met substitution) were active.
The yeast and human BPLs are of similar length (690 and 726 residues, respectively) and share weak sequence similarity in the N-terminal half of the protein. Unlike our findings, Polyak et al. (43) have shown an absolute dependence of yeast BPL on inclusion of the N-terminal domain for biotinylating activity, demonstrated using N-terminal deletions and sensitivity of the enzyme to protease cleavage. Significantly, these authors identified a protease sensitive site in yeast BPL, which they propose acts as a hinge region that brings together the two halves of the protein upon biotin binding. This is similar to our conjecture about human HCS. The difference compared with our results may lie in instability of the truncated products of yeast BPL or perhaps that biotin binding, in the absence of the N terminus, is too weak to catalyze significant product formation. The linker region identified in the yeast BPL spans residues Lys-240-Asn-260, which corresponds approximately to Lys-312-Glu-336 (with a four-residue gap included). This region is conveniently located between the biotinylation domain (Gly-466-Val-674) and the Leu-166-Arg-290 N-terminal domain that we identified in the human enzyme. The location of this putative linker region provides an explanation for the results obtained for the human HSC deletion constructs. The shortest HCS constructs that retain biotinylating activity, Arg-290, Pro-338, and Lys-378, all have their N terminus in the sequence surrounding the linker region. Thus, removal of the N-terminal domain up to the linker region results in a stable, functional protein. Indeed, the construct showing the highest level of protein by Western blot is Lys-378, which has its N terminus beyond the carboxyl end of the putative linker region.
A significant property of the truncated human HCS was its differing behavior toward the BCCP, BCCP87, and p-67 acceptor substrates. The complementation assay tested the ability of the constructs to biotinylate BCCP at levels sufficient to permit growth of birA104, and these results were substantiated in the crude extract assays, which measured the biotinylation of remaining BCCP and the coexpressed p-67 substrate. Whereas the longest HCS, starting at Met-58 or Ala-80, were active toward both p-67 and BCCP, Arg-290 and Pro-338 showed a clear bias toward BCCP, with p-67 biotinylation essentially undetectable in the assay. The activity toward both substrates was restored in Lys-378. In the kinetically more interpretable assays using purified enzyme to assay equimolar mixtures of BCCP87 and p-67 (Fig. 5), Met-58 and Ala-80 were similarly active toward the two substrates. In contrast, Arg-290 and Pro-338 showed weak but significant activity toward p-67 but only trace activity toward BCCP87. Similarly, purified Lys-378 also showed a greater affinity for p-67 compared with BCCP87. The lower overall activity of Arg-290 and Pro-338 compared with Lys-378 is explained by the Western blot, which shows less protein in the assay than found for Lys-378. The disparity between the biotinylation of BCCP and BCCP87 by the significantly truncated HCS versus the near full-length HCS is more difficult to explain. It is possible that the N terminus of HCS participates in the interaction with the acceptor substrate, so that any difference in the interaction with BCCP and BCCP87 might become pronounced in the more extensively truncated HCS. However, this conjecture contrasts with the absence of any discernible difference in the rate of biotin transfer to the two substrates by BirA (44). These results, implicating N-terminal interaction with the acceptor substrates, call for dissection of the two half-reactions governing biotin transfer to apocarboxylase substrates.
Whereas eukaryotic and prokaryotic BPLs share an essentially identical biotinylation activity, they have completely distinct N-terminal sequences. In E. coli, the N terminus contains the biotin operon repressor function of BirA. Its corepressor is biotin-AMP, the product of the first half-reaction in the biotinylation of BCCP. When all of the available apo-BCCP becomes biotinylated, newly synthesized biotin-AMP remains associated with BirA and the BirA·biotin·AMP complex accumulates and binds to the operator sequence of the biotin operon, thereby repressing further transcription of the biotin biosynthetic genes. Beckett and co-workers (45, 46) have shown that biotin and biotin-AMP binding to BirA induces large conformational changes in the complex and Wilson et al. (13) showed that addition of biotin or biotin-AMP to crystallized BirA resulted in destruction of the crystals. These data pointed to the critical involvement of the N-terminal domain in tight binding of biotin and biotin-AMP. Xu and Beckett (46) further showed that deletion of the N terminus dramatically reduced the affinity for biotin and biotin-AMP without reducing the maximal rate of biotin-AMP synthesis. They also showed that the dissociation of the BirA·biotin·AMP complex occurs 100 times faster in the truncated protein than full-length BirA. It is not evident whether the molecular basis for the involvement of the N terminus in eukaryotic BPLs is similar. Because the sequences are unrelated, the parallels between these interactions may be coincidental. Alternatively, perhaps eukaryotic BPLs have evolved a related but biochemically distinct role in gene action in eukaryotic cells. To this end, there are several reports of biotin-mediated regulation of transcription or translation of mammalian genes (47-51).
Our results provide an alternate explanation for the biotin responsiveness of HCS-deficient patients with mutations outside the biotin binding region. For patients with mutations within the biotin binding region, their biotin responsiveness can be explained because at least one allele expresses mutant enzyme with an elevated Km for biotin (35-37). However, for patients with both alleles mapping outside the biotin binding region, or where the second allele is nonexpressing, their biotin responsiveness has been less easy to explain. One suggestion is based on mass action; plasma biotin levels are so far below the Km of the enzyme that any increase in biotin levels, afforded by high dose treatment with biotin, would result in an increase in HCS activity as long as there remained any unoccupied enzyme (35-37). Whereas this option remains plausible, our results, in combination with the findings for yeast BPL, provide a rationale for biotin responsiveness that takes into account the effect of biotin on the integrity of the enzyme. Three of these point mutations (R183P, L216R, L237P) are found within the region defined by the N-terminal domain Leu-166-Arg-290, described above (Fig. 1). Two others, V333E and V363D, are in the vicinity of the proposed linker sequence or within the sequence defined by the functional, truncated proteins. In these cases, the biotin responsiveness of patients may be associated with a biotin-mediated stabilization of the substrate-bound complex.
Our studies raise a caution for the analysis of HCS activity from
patients with multiple carboxylase deficiency where BCCP is used as the
substrate (35, 37, 52). The implication for varying impact of the N
terminus of HCS in biotin transfer, including in the interaction with
the peptide substrate, suggests that natural substrates should be
favored for diagnostic use. Apocarboxylase fragments such as p-67, from
human propionyl-CoA carboxylase, or p-86 from pyruvate carboxylase (7)
may prove to be more informative of the functional state of mutant
human enzyme.
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FOOTNOTES |
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* This work was supported by a grant from the Medical Research Council of Canada.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Present address: Lawrence Berkeley National Laboratory, Life
Sciences Division, MS74-157, 1 Cyclotron Rd., Berkeley, CA 94720.
§ To whom correspondence should be addressed: Department of Cell Biology and Anatomy, University of Calgary, Room 250 Heritage Medical Research Bldg., 3330 Hospital Dr. N.W., Calgary, Alberta T2N 4N1. Tel.: 403-220-2268; Fax: 403-210-8115; Email: rgravel@ucalgary.ca.
Published, JBC Papers in Press, December 21, 2000, DOI 10.1074/jbc.M009717200
2 E. Campeau and R. Gravel, manuscript in preparation.
3 L. Del Rio and R. Gravel, unpublished results.
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ABBREVIATIONS |
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The abbreviations used are:
BPL, biotin protein
ligase;
BCCP, biotin carboxyl carrier protein;
HCS, holocarboxylase
synthetase;
HCS deficiency, multiple carboxylase deficiency;
IPTG, isopropyl-1-thio--D-galactopyranoside;
PCR, polymerase
chain reaction;
NTA, nitrilotriacetic acid;
LB, Luria-Bertani.
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