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Journal of Bacteriology, January 1999, p. 347-352, Vol. 181, No. 1
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
APT1, but Not APT2, Codes for
a Functional Adenine Phosphoribosyltransferase in
Saccharomyces cerevisiae
Juan D.
Alfonzo,1,
Timothy R.
Crother,1
Maria L.
Guetsova,2
Bertrand
Daignan-Fornier,2 and
Milton W.
Taylor1,*
Department of Biology, Indiana University,
Bloomington, Indiana 47405,1 and
Institut de Biochimie et Genetique Cellulaires, Bordeaux,
France2
Received 18 August 1998/Accepted 21 October 1998
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ABSTRACT |
The yeast Saccharomyces cerevisiae has two separate
genes (APT1 and APT2) that encode two
potentially different forms of adenine phosphoribosyltransferase
(APRT). However, genetic analysis indicated that only APT1
could code for a complementing activity. Cloning and expression of both
the APT1 and APT2 genes in Escherichia coli showed that although discrete proteins (APRT1 and APRT2) were made by these genes, only APRT1 had detectable APRT activity. Northern and Western blot analyses demonstrated that only
APT1 was transcribed and translated under normal
physiological conditions in yeast. Phylogenetic analysis revealed that
APRT1 and APRT2 are evolutionary closely related and that they arise
from a gene duplication event. We conclude that APT1 is the
functional gene in S. cerevisiae and that APT2
is a pseudogene.
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TEXT |
In most organisms, purine
nucleotides can be synthesized de novo by a series of 10 enzymatic
reactions that lead to the formation of IMP (4, 5, 20). IMP
can be further converted to AMP or GMP to satisfy the purine nucleotide
requirements of a growing cell. Alternatively, free-purine bases can be
directly recycled from the growth medium and incorporated into purine
nucleotide pools. Both sets of reactions involve the action of
phosphoribosyltransferases (PRTases), a group of enzymes that have in
common the chemistry of transferring the ribose 5-phosphate from
-D-5-phosphoribosyl 1-pyrophosphate (PRPP) onto a
nitrogenous base to form an N-riboside monophosphate and
pyrophosphate (20). PRTases are essential not only for
purine biosynthesis but also for the biosynthesis of pyrimidines,
pyridines, histidine, and tryptophan (20).
Adenine PRTase (APRT) is the key enzyme in the direct recycling of free
adenine into purine nucleotide pools. APRT catalyzes the
Mg2+-dependent transfer of the phosphoribosyl group from
PRPP to adenine to form the nucleotide AMP (2, 4, 8, 11, 14, 16, 19, 21, 28, 30). In humans, APRT deficiency causes the accumulation of a poorly soluble adenine derivative, 2,8-dihydroxy adenine, which leads to urolithiasis and renal failure (27).
Typically, APRTs are encoded by constitutively expressed single-copy
genes (22). However, two genes encoding two forms of APRT in
Arabidopsis thaliana that differ in their nucleotide
specificities have recently been reported (18, 25). We have
previously identified a gene coding for APRT in Saccharomyces
cerevisiae (APT1) (2). In addition, Yuryev
and Corden reported the sequence of another potential APT
gene in yeast (APT2), based on sequence comparison analysis
(32). The finding of two different genes that may encode APRT in yeast has led us to propose that more than one form of this
enzyme may also occur in yeast.
To help understand the relationship between APT1 and
APT2 and address the possibility that two forms of the
enzyme also occur in S. cerevisiae, both genes were used in
complementation studies with yeast mutants deficient in APRT activity.
Mutations disrupting APT1 and APT2 were made.
Whereas disruption of APT1 eliminated APRT activity,
disruption of APT2 had no effect on APRT activity or
repression of de novo purine biosynthesis by adenine. Both genes were
also individually expressed in Escherichia coli cells. Expression of a recombinant APT2 showed that this gene is
defective in that it does not encode a functional APRT enzyme. From the complementation and expression studies, evidence is presented to
support the hypothesis that APT1 is required and by itself sufficient to code for APRT in S. cerevisiae. In addition,
the data presented here lead us to propose that APT2 is in
fact a pseudogene, derived from a gene duplication event.
Strains, plasmids, and culture conditions.
E. coli NM522
(GIBCO-BRL) was grown on 2× YT medium supplemented with ampicillin (50 µg/ml of culture) for routine growth of plasmids. E. coli
B25 and B26, used in the high-level expression of the APT1
and APT2 genes, were grown on similar medium but also supplemented with kanamycin to select for the lacZ-repressor
plasmid, as described in the Qiagen manual.
The following yeast strains were used in this study: Y642 (MAT
ura3-52 leu2-3,112 lys2
201 his3200
trp1::hisG) (this study), Y643
(MATa ura3-52 leu2-3,112 lys2201
his3200 trp1::hisG) (this study), L3852
(MAT ade2 his3200 leu2-3,112 lys2201
ura3-52) (G. Fink), L4364 (MATa ade2 his3200
leu2-3,112 lys2201 ura3-52) (G. Fink), Y810
(MAT ura3-52 leu2-3,112 lys2201 his3200 trp1::hisG apt2::HIS3)
(this study), Y812 (MATa ura3-52 leu2-3,112 lys2201 his3200
trp1::hisG apt2::HIS3)
(this study), Y814 (MAT ade2 ihs3200 leu2-3,112
lys2201 ura3-52 apt2::HIS3) (this study),
Y808 (MATa ade2 his3200 leu2-3,112
lys2201 ura3-52 apt2::HIS3) (this study),
W109-9C (MATa ade2 trp1 ura3 his3 hpt1-27) (R. Woods), DS1.2B/1 (MAT ade2 apt1 aah1 ura3) (R. Woods), Y839 (MATa ura3-52 leu2-3,112
lys2201 his3200 apt2::HIS3
hpt1::URA3) (this study), Y511
(MATa ura3 lys2 leu2
apt1::URA3) (B. Daignan-Fornier), Y350
(MATa ura3 lys3 leu2) (B. Daignan-Fornier), Y842
(MATa ura3-52 leu2-3,112 lys2201
his3200 trp1::hisG
apt2::HIS3 aah1::URA3) (this
study), X79 (MATa leu2-1 trp1-1) (R. Woods),
Y382 (MATa ade2 ade3 ura3 leu2 trp1) (A. Bender), Y388 (MATa ade2 ade3 ura3 leu3 lys1)
(A. Bender), Y839 (MATa ura3 trp1 leu2 his3
pep::His3 prb1 can1 GAL) (A. Bender), Y847
(MATa ura3-52 leu2-3,112 lys2201
his3200 apt2::HIS3
apt1::URA3) (this study), and MWT32
(MATa leu2 ade2 ade3 apt1) (M. Taylor).
Yeast cells were transformed by the lithium chloride-triacetin method
(
17). Bacterial transformations were carried out by
the
MnCl
2 method (
24).
Complementation and genetic analysis of APRT.
Transformants
were selected by complementation of the URA mutation to the
URA+ phenotype (by the plasmid-derived URA
marker) in strain DS1.2B and scored for their ability to use adenine as
the sole source of purine. Both the APT1 (pRSAPT1, single
copy) and APT2 (pRSAPT2, single copy) genes were
individually transformed into the DS1.2B mutant and tested for
complementation. The APT1 gene complemented the
APT mutant phenotype, allowing the APRT-deficient mutant
DS1.2B to grow on defined media containing adenine as the sole purine source. The APT2 gene (12) failed to complement
the DS1.2B mutant (Table 1). Also, as
shown in Table 1, only APT1-transformed cells had wild-type
levels of APRT activity.
The
APT2 gene was disrupted by replacing its entire coding
region with the
HIS3 gene (
6). The resulting
plasmid, named
P878, carrying the
apt2::
HIS3 construct was amplified with
the
following synthetic oligonucleotides: APT23,
5'-GCTACTGTGCATACCGC-3',
and APT24,
5'-GAGGCACTTTGAACGGC-3'. The resulting PCR product
was used
to transform the yeast strains Y642, Y643, L3852, and
L4364.
Transformants were selected for histidine prototrophy.
Correct
integration was verified by PCR. Disruption of the
APT2 gene
in a wild-type strain does not lead to any obvious growth
phenotype.
Since
apt1 mutants were previously shown to be resistant
to
8-azaadenine (
23), we tested the resistance of the
apt2-disrupted
strains to this base analog. We found that
the
apt2 mutant is
as sensitive to 8-azaadenine as the
isogenic wild-type strain.
Furthermore, the
ade2 apt2 double
mutant (where the
ade2 mutation
blocks de novo purine
biosynthesis) can use adenine or hypoxanthine
as a purine
source.
Mutations affecting purine salvage also inhibit adenine repression of
the genes encoding enzymes of the purine de novo pathway
(
7). We have therefore tested whether the
apt2-disrupted strain
was affected in this regulation
process. Expression of an
ADE1 (
N-succinyl-5-aminoimidazole-4-carboxamide ribotide
synthetase,
a purine de novo enzyme)-
lacZ fusion was assayed
in the
apt2 mutant
and isogenic wild-type strains. The
apt2 mutation has no effect
on adenine repression of the
ADE1-lacZ fusion.
apt2 aah1,
apt2 hpt1, and
apt1 apt2
double mutants were constructed. All the double mutants grew normally
and were phenotypically
indistinguishable from the isogenic single
mutants in a wild-type
APT2 background.
apt1 apt2
double mutants salvaged adenine through
adenine aminohydrolase. All
together, these results suggest that
apt2 disruption does
not severely affect purine utilization during
vegetative
growth.
To test whether
APT2 encodes a minor isoform of APRT, we
introduced the
APT2 gene on a multicopy vector (P552)
(
12,
29)
into an
apt1 aah1 ade2 triple mutant.
This strain is unable to
use adenine as a purine source but grows
normally through conversion
of hypoxanthine into IMP by
hypoxanthine-guanine phosphoribosyl
transferase. The multicopy vector
carrying the
APT2 gene is unable
to restore adenine
utilization to the triple mutant strain, showing
that even when
overexpressed,
APT2 is unable to compensate for
the lack of
APT1. Similarly, overexpression of
APT2 does not
restore
utilization of hypoxanthine in an
hpt1 ade2 double
mutant, thus
indicating that APRT2 has no significant hypoxanthine
PRTase
activity.
Our finding that
APT1, but not
APT2, could
complement an APRT-deficient mutant suggests that either
APT2 does not encode a
functional APRT or that
APT2 is indeed required for APRT activity
but that it is not
by itself sufficient to encode a functional
enzyme. However, the fact
that disruption of the
APT2 gene had
no effect on adenine
utilization, adenine analog resistance, or
regulation of de novo purine
biosynthesis further supports the
view that APRT2 serves no function in
purine recycling in
S. cerevisiae.
Expression of recombinant APRT1 and APRT2 proteins.
The
APT1 and APT2 genes were individually ligated
into His-tag expression vectors (Qiagen, Hilden, Germany), and the
pQEAPT1 and pQEAPT2 expression constructs, respectively, were
generated. These constructs allow for the expression of the recombinant
APRT1 and APRT2 proteins in E. coli with an N-terminal
hexahistidine tag. To express the APRT1 and APRT2 proteins, E. coli B25 (Qiagen) was individually transformed with each construct
(pQEAPT1 or pQEAPT2) and cells were grown as described in the Qiagen
manual. Cells (1L) were routinely grown to mid-log phase
(A600, ~0.5) at 37°C, the point at which
IPTG (isopropyl-
-D-thiogalactopyranoside) was added to a
final concentration of 1 mM. The cells were grown for five additional
hours after IPTG addition.
E. coli cells expressing
APT1 and
APT2
were harvested by centrifugation at 5,000 ×
g in a
Sorvall centrifuge at 4°C for 15
min. The cells were suspended in 30 ml of sonication buffer (50
mM Tris-Cl [pH 7.4], 5 mM
MgCl
2, 20 mM KCl) and broken by sonication
at maximum power
with a microtip for cycles of 1 min with a 1-min
rest for a total of 10 min. The resulting extract was spun at
20,000 ×
g for
30 min, and the resulting cell extract was gravity
loaded onto a 2-ml
Ni
2+-nitrilotriacetic acid column. The column was washed
with 10 column
volumes of sonication buffer (20 ml) containing 50 mM
imidazole
and eluted with 4 column volumes of the same buffer
containing
150 mM imidazole, as described in the Qiagen protein
expression
manual. The
APT1 and
APT2 genes were
inserted in plasmid vectors
under the control of an IPTG-inducible
promoter and expressed
in
E. coli cells (Qiagen). The
APT1 gene product (APRT1) migrated
as a 25-kDa band, and the
APT2 gene product (APRT2) migrated as
26-kDa band in a
sodium dodecyl sulfate-12.5% polyacrylamide gel
(Fig.
1). These sizes are in agreement with the
sizes expected
from the deduced coding sequences of the two genes with
the His
tag at their N termini.
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FIG. 1.
Expression of hexahistidine-tagged APRT1 and APRT2
proteins in E. coli cells. Lane 1, total cell extract from
E. coli cells transformed with the His-tagged
APT1 gene; lane 2, Ni2+-purified recombinant
APRT1 protein; lane 3, total cell extract from E. coli cells
transformed with the His-tagged APT2 gene; lane 4, Ni2+-purified recombinant APRT2 protein; lanes 5 and 6, purified recombinant APRT1 and APRT2 proteins (respectively) run next
to each other to emphasize their relative size difference.
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In order to assess the sizes of APRT1 and APRT2 in solution, both
recombinant proteins were separately loaded onto a Sephadex
G-200
column, calibrated with protein standards, and developed
as previously
described (
1a) (Fig.
2). The
purified APRT1 and
APRT2 proteins were individually loaded, and the
column was developed
with the equilibration buffer. Five-milliliter
fractions were
collected, and their relative protein contents were
estimated
by measurements of optical density at 280 nm with a model 160
UV spectrophotometer (Shimadzu). Protein-containing fractions
were
assayed for APRT activity by measuring the incorporation
of
3H-labeled adenine into AMP, after the enzyme fraction to
be tested
was incubated with PRPP and [
3H]adenine in the
appropriate buffer (
15). The fraction with
the highest APRT
activity (100% relative activity) was used as
the peak fraction for
determining the native size of the enzyme
in solution.
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FIG. 2.
Sizing of the APRT1 and APRT2 recombinant proteins. (A)
His-tagged APRT1 was chromatographed on a Sephadex G-200 column as
described in Materials and Methods. The peak of activity corresponds to
that of a 50-kDa protein. (B) The His-tagged APRT2 protein was
chromatographed through the same Sephadex column. As no APRT activity
was detected with this protein, the peak of absorbance (optical density
at 280 nm [O.D.280]) is given and corresponds to that of a 26-kDa
protein. -Amylase (200 kDa), bovine serum albumin (BSA; 66 kDa),
carbonic anhydrase (29 kDa), and cytochrome c (cyt C; 13 kDa) were used as standards to calibrate the column. vo, void volume;
vt, total volume.
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APRT1 eluted between the bovine serum albumin (66 kDa) and carbonic
anhydrase (29 kDa) standards. The peak of activity observed
coincided
with the molecular mass of a 50-kDa protein (Fig.
2A).
This molecular
mass agrees with that of a homodimer of 25-kDa
subunits. When APRT2 was
chromatographed through the same column,
it eluted in a fraction
lacking any detectable APRT activity.
The peak of absorbance
(
A280) corresponded to a 25-kDa protein
(Fig.
2B); thus, APRT2 failed to dimerize. The finding that the
APRT1 protein
had enzymatic activity comparable to that of the
native enzyme
previously purified in our laboratory suggests that
indeed the
APT1 gene is sufficient to code for a functional enzyme.
Our
failure to detect any activity associated with the recombinant
APRT2
protein led us to conclude that either the
APT2 gene does
not encode a functional enzyme or the recombinant APRT2 expressed
in
E. coli does not fold into a catalytically active
conformation.
The failure of APRT2 to dimerize when it was separated
through
a sizing column suggested that the lack of APRT2 activity is
due,
in part, to its failure to dimerize. In fact, all of the
previously
characterized APRTs (from mouse, hamster, human,
E. coli, and
Arabidopsis cells), with the exception of
Leishmania donovani APRT (
30), are functional as
homodimers in solution (
20).
This failure to dimerize may
also be due to improper folding of
E. coli-expressed APRT2.
However, given the degree of sequence
similarity between the two genes
(
1a), the latter explanation
seems unlikely. In addition,
high-level expression of
APT2 in
the APRT-deficient Y847
strain showed no APRT activity (
6b).
Analysis of APRT expression.
Total RNA was isolated from
various yeast strains by the acid-phenol method (13). For
Northern blot analysis, poly(A)+ RNA (5 µg) from strain
Y382 or X79 was separated by electrophoresis in a 18%
formaldehyde-1.2% agarose gel (Seakem). The gel was run at 100 V for
4 h. The RNA was transferred by means of capillarity to a
Zeta-probe membrane as described in the Bio-Rad manual. The membrane
was hybridized to the radiolabeled APT1 and/or
APT2 probe as described in the Zeta-probe manual. The
membrane was exposed to X-ray film (Kodak) for 16 h and developed
in an X-Omat machine (Kodak).
Western blot analyses were carried out with cell extracts from various
yeast strains, prepared by disruption with glass beads.
Samples were
electrophoretically separated in a sodium dodecyl
sulfate-12%
polyacrylamide gel. The proteins were transferred
to Trans-Blot
transfer membranes by electrophoresis as described
in the Bio-Rad
manual. Membranes were blocked with 5% nonfat milk
(to prevent
nonspecific binding of the antibody), and the blots
were separately
probed with rabbit anti-APRT1 or rabbit anti-APRT2
polyclonal
antibodies. For detection, a horseradish peroxidase-linked
secondary
antibody (Bio-Rad) was hybridized to the same membrane.
Bands were
visualized by chemiluminescense with an Immuno-Star
kit (Bio-Rad). The
membrane was exposed to X-ray film, and the
film was developed in an
X-Omat machine
(Kodak).
We observed that both the
APT1 and
APT2 genes
were actively transcribed in wild-type yeast cells. However, we failed
to detect
any APRT2 protein in Western blot experiments using extracts
from
wild-type yeast and polyclonal antibodies against the recombinant
APRT2 protein (Fig.
3B). When similar
experiments were carried
out with anti-APRT1 antibodies, we could
easily detect an APRT1
signal (Fig.
3A). As previously mentioned, the
APRT2 protein could
still be made but quickly degraded. Regardless, the
failure to
detect activity and/or the presence of a protein
corresponding
to APRT2 argues that the bulk of the APRT activity in
vivo is
provided by
APT1 gene expression. These data also
suggest that
the
APT2 gene product either lacks elements
important for efficient
translation or lacks elements important for
proper protein folding
and/or stability in vivo. However,
overproduction of APRT2 in
E. coli and yeast results in a
stable nonactive protein (
6a).
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FIG. 3.
Western blot analysis of native APRT proteins. (A)
Western blot probed with polyclonal anti-APRT1 antibody. Lane 1 contains a cell extract from strain Y350 (wild-type strain), lane 2 contains a cell extract from strain Y511 (apt1 mutant
strain), and lane 3 contains pure recombinant APRT1. (B) Western blot
similar to that shown in panel A but probed with polyclonal anti-APRT2
antibody. Lanes 1 and 2 contain cell extracts from strains Y350 and
Y511 (respectively), and lane 3 contains pure recombinant APRT2.
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We have hypothesized (
1) that the role of the APRT2 protein
is to interact with APRT1, thus down-regulating its activity
and/or
specificity. High levels of purine nucleotides can lead
to repression
of the de novo purine biosynthetic pathway. We hypothesized
that the
APRT1-APRT2 interaction would be particularly important
during
conditions of starvation (i.e., depletion of free adenine),
where APRT
activity becomes less important as the cell is forced
to synthesize
purine bases de novo. This hypothesis predicts that
the levels of APRT2
transcripts increase as cells deplete free
adenine from the medium
(i.e., as cells enter stationary phase).
However, when Northern blot
analysis was performed with radiolabeled
DNA probes specific for
APT1 or
APT2, we detected comparable levels
of
APT1 and
APT2 transcription in wild-type cells
regardless of
the growth phase of the culture (Fig.
4).
APT2 mRNA migrates
slightly
more slowly than
APT1 mRNA. These experiments
demonstrate that
even if the
APT2 gene is actively
transcribed, at least under
the culture conditions described, it is not
actively translated
(Fig.
3).
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FIG. 4.
Northern blot analysis of the APT1 and
APT2 gene products from strain X79 (wild type). (A) Total
RNA was extracted at various times during growth and probed with a
radiolabeled APT1 probe. (B) Same membrane as that shown in
panel A, probed with a radiolabeled APT2 probe. (C) Same
membrane as that shown in panel A, probed with a radiolabeled yeast
actin used as a loading control.
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Phylogenetic comparison analysis of the APRT1 and APRT2
proteins.
Amino acid sequence alignments obtained from the SeqApp
program were used in the PAUP program (version 3.11; Smithsonian) to
determine the phylogenetic relationship between various APRTs. The
analysis was performed by maximum parsimony analysis with the
exhaustive-search method. Bacterial sequences were used as outgroups.
The S. cerevisiae APRT1 (GenBank accession no. S49755) and
APRT2 (GenBank accession no. L14434) sequences were used in the
alignment, together with the homologous APRTs (GenBank accession
numbers in parentheses) from E. coli (M14040),
Haemophilus influenza (U32748), Drosophila
melanogaster (S34831), D. pseudoobscura AF025800),
Mus musculus (M86440), Homo sapiens (p07741),
Caenorhabditis elegans (U80438), and Arabidopsis thaliana APRT1 (p31166). The phylogenetic analysis was performed on the APRT sequence alignment previously described by us
(1a) (Fig. 5). We wished to
determine if APT2 was the result of a duplication of
APT1 (or vice versa) or if APT2 was more closely
related to some other APRT. The phylogenetic analysis showed that
APT1 is most closely related to APT2.
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FIG. 5.
Comparative phylogenetic reconstruction of APRT1 and
APRT2. A phylogenetic tree of various deduced APRT sequences
constructed with PAUP version 3.11 is shown. Numbers indicate the
probability of two sequences branching together.
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Upon completion of the Yeast Genome Project, it was discovered that
much of the genome was in fact duplicated. Fifty-five
duplicate regions
which cover approximately 50% of the
S. cerevisiae genome
have been found (
10). It has been proposed that the entire
yeast genome was duplicated and that subsequently many of the
duplicated regions were lost (
31).
APT1 and
APT2 are both found
in duplicated regions of each other:
APT1 on chromosome XIII and
APT2 on chromosome IV
(
31). Southern blot analysis was used
to determine if this
APT duplication event was found only in
S. cerevisiae. The closely related yeast
Picchia
pastoris was examined
for the presence of two
APTs.
With
APT1 and
APT2 probes, it appears
that
P. pastoris also contains two
APTs
(data not
shown).
Taken together, the complementation and the expression data lead us to
conclude that
APT1 is by itself sufficient to code
for APRT
in
S. cerevisiae. Furthermore, from the phylogenetic
comparative analysis, we propose that the
APT2 gene is
a pseudogene,
perhaps derived from an aberrant gene duplication
of the
APT1 gene. The occurrence of pseudogenes in yeast,
although rare, is
not unprecendented. It is possible that
APT2 codes for an APRT
homolog that has diverged to the
point of possessing a different
function. However, our failure to
detect APRT2 protein in various
yeast strains makes this possibility
unlikely and makes our original
proposal of two forms of APRT in yeast
untenable.
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ACKNOWLEDGMENTS |
We are grateful to Alan Bender, J. L. Corden, G. Fink, and R. Woods for sending plasmids and strains.
This work was supported by grants from the Fondation pour la Recherche
Medicale, Conseil Regional d'Aquitaine, and the CNRS (UPR9026). M.L.G.
was supported by a Ministère des Affaire Etrangères fellowship.
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FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Biology, Indiana University, Bloomington, IN 47405. Phone: (812)
855-3340. Fax: (812) 855-6705. E-mail: taylor{at}indiana.edu.
Present address: Howard Hughes Medical Institute, MacDonald
Research Laboratories, University of California at Los Angeles, Los
Angeles, CA 90024.
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Journal of Bacteriology, January 1999, p. 347-352, Vol. 181, No. 1
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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Abstract
Text
mutant
transformed with the APT1 and
APT2 genesa
