From the a Department of Genetics, In the present studies, we show that the SecD and
SecF equivalents of the Gram-positive bacterium Bacillus
subtilis are jointly present in one polypeptide, denoted SecDF,
that is required to maintain a high capacity for protein secretion.
Unlike the SecD subunit of the pre-protein translocase of
Escherichia coli, SecDF of B. subtilis was not
required for the release of a mature secretory protein from the
membrane, indicating that SecDF is involved in earlier translocation
steps. Strains lacking intact SecDF showed a cold-sensitive phenotype,
which was exacerbated by high level production of secretory proteins,
indicating that protein translocation in B. subtilis is
intrinsically cold-sensitive. Comparison with SecD and SecF proteins
from other organisms revealed the presence of 10 conserved regions in
SecDF, some of which appear to be important for SecDF function.
Interestingly, the SecDF protein of B. subtilis has 12 putative transmembrane domains. Thus, SecDF does not only show sequence
similarity but also structural similarity to secondary solute
transporters. Our data suggest that SecDF of B. subtilis represents a novel type of the SecD and SecF proteins, which seems to
be present in at least two other organisms.
The translocation of proteins across biological membranes involves
the action of complex machineries, consisting of at least two
functional units as follows: a force generator (motor) and a
translocation channel (1). Escherichia coli is the best
characterized of the eubacterial protein translocation machineries. The
so-called pre-protein translocase of E. coli consists of at
least seven proteins as follows: SecA, SecD, SecE, SecF, SecG, SecY,
and YajC. SecA is a peripheral membrane protein, which generates the
driving force for the initiation of precursor transport through the
translocation channel, of which SecY, SecE, and SecG are the most
important components. Recent studies suggest that SecY, SecE, and SecG
form a heterotrimeric subcomplex (SecYEG) of a large "holoenzyme," which also contains a heterotrimeric subcomplex of SecD, SecF, and YajC
(SecDFyajC; see Refs. 2 and 3). Once protein translocation is initiated
by SecA, further translocation is driven both by SecA and the proton
motive force (PMF1; Refs.
4-6). Current models suggest that SecA drives protein transport
through cycles of pre-protein binding, membrane insertion, pre-protein
release, and deinsertion from the membrane (7, 8). The cycling of SecA
is regulated by ATP binding and hydrolysis, which causes major
conformational changes in this protein (9, 10).
The role of SecDFyajC in protein translocation in E. coli is
not completely clear, in particular because it is not essential for
protein translocation in vitro (11) and because SecD and SecF are required to maintain a stable PMF (12). Moreover, SecDFyajC seems to be involved in at least three aspects of the translocation process: first, the cycling of SecA is modulated by SecDFyajC, which
stabilizes the membrane-inserted state of SecA (8, 13-15); second,
SecDFyajC seems to stimulate PMF-driven protein translocation (15); and
third, SecD appears to be required for the release of mature proteins
from the extracytoplasmic side of the membrane (16). Thus, SecDFyajC
may have an indirect role in protein translocation in E. coli, for example in the assembly of the protein translocase complex, the gating of the translocation channel (17), or the stimulation of PMF-driven protein translocation (15).
Although homologues of SecD and SecF of E. coli have been
identified in several eubacteria and archaea (17), their role in
protein translocation has not been addressed experimentally. In the
present studies, we have investigated the role of the SecD and SecF
equivalents in the Gram-positive bacterium Bacillus
subtilis, which is a particularly suitable organism for this
purpose: first, B. subtilis secretes proteins into the
growth medium directly after translocation across the membrane (see
Ref. 18); second, the capacity for protein secretion can be probed
under conditions of hypersecretion (19); third, important components of
the protein translocation machinery of B. subtilis, such as
SecA, SecY, and SecE, have been identified (20-23); and fourth, the
gene for a SecF-like protein was recently identified by genome
sequencing (24). Interestingly, unlike the secF genes from
E. coli and other well characterized microorganisms, the
secF-like gene of B. subtilis seemed to represent
a natural gene fusion between the equivalents of secD and
secF. The results of our studies show that the SecD and SecF
equivalents of B. subtilis are indeed jointly present in one
polypeptide, which is required for efficient translocation of secretory
pre-proteins under conditions of hypersecretion.
Plasmids, Bacterial Strains, and
Media--
Table I lists the plasmids
and bacterial strains used. TY medium and the S7 media 1 and 3, for the
pulse-labeling of B. subtilis, were prepared as described in
Ref. 25, with the exception that in S7 media glucose was replaced by
maltose. Minimal medium (GCHE medium) was prepared as described in Ref.
26. Antibiotics were used in the following concentrations:
chloramphenicol, 5 µg/ml; erythromycin, 1 µg/ml; kanamycin, 10 µg/ml; ampicillin, 50 µg/ml. IPTG was used at 1 mM.
ABSTRACT
Top
Abstract
Introduction
Procedures
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Procedures
Results
Discussion
References
EXPERIMENTAL PROCEDURES
Top
Abstract
Introduction
Procedures
Results
Discussion
References
Plasmids and bacterial strains
DNA Techniques--
DNA techniques and transformation of
competent E. coli DH5 cells were carried out as described
in Ref. 27. Enzymes were from Boehringer Mannheim (Mannheim, Germany).
B. subtilis was transformed as described in Ref. 26. The
sequences of primers used for PCR (5'-3') are listed below;
nucleotides identical to genomic template DNA are printed in capital
letters and restriction sites used for cloning are underlined. DNA
sequences were determined as described in Ref. 28.
Pulse-Chase Protein Labeling, Immunoprecipitation, SDS-PAGE, and Fluorography-- Pulse-chase labeling experiments with B. subtilis, immunoprecipitations, and SDS-PAGE were performed as described in Ref. 25. Fluorography was performed with Autofluor (National Diagnostics, Atlanta, GA). Relative amounts of precursor and mature forms of secreted proteins were estimated by scanning of autoradiographs with a laser densitometer (LKB, Bromma, Sweden).
Western Blot Analysis-- Western blotting was performed using a semi-dry system as described in Ref. 29. After separation by SDS-PAGE, proteins were transferred to Immobilon-polyvinylidene difluoride membranes (Millipore, Bedford, MA). Proteins were visualized with specific antibodies and horseradish peroxidase anti-rabbit or anti-mouse IgG conjugates, using the ECL detection system of Amersham (Little Chalfont, UK). Streptavidin-horseradish peroxidase conjugate was obtained from Amersham Pharmacia Biotech.
Protease Accessibility-- Protoplasts were prepared from exponentially growing cells of B. subtilis. Cells were concentrated 5-fold in protoplast buffer (20 mM potassium phosphate, pH 7.5; 15 mM MgCl2; 20% sucrose) and incubated for 30 min with 1 mg/ml lysozyme (37 °C). Protoplasts were collected by centrifugation, resuspended in fresh protoplast buffer, and incubated at 37 °C in the presence of 1 mg/ml trypsin (Sigma) for various periods. The reaction was terminated by the addition of 1.2 mg/ml trypsin inhibitor (Sigma). Finally, protoplasts were collected by centrifugation and analyzed by SDS-PAGE and Western blotting. In parallel, protoplasts were incubated without trypsin, or in the presence of trypsin and 1% Triton X-100. Samples containing Triton X-100 were directly used for SDS-PAGE after the addition of trypsin inhibitor.
-Galactosidase Activity--
The
-galactosidase assay and
the calculation of
-galactosidase units (per
A600) were performed as described in Ref.
30.
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RESULTS |
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Identification of the secDF Gene of B. subtilis-- The remarkable observation that the secD and secF genes of B. subtilis might be present in one open reading frame was tested and confirmed to be correct by cloning and resequencing the genomic region comprising the secF-like gene. Therefore, we renamed the secF-like gene secDF. Because a few errors were detected in the published sequence (GenBankTM accession number g2635229; Ref. 24), the corrected sequence was submitted to the GenBankTM data base. The secD operon of E. coli consists of the yajC, secD, and secF genes (31). This function-related operon structure is not conserved in B. subtilis, as the yajC-like gene yrbF and secDF are separated by two pairs of divergently transcribed genes (Fig. 1A). Like yajC of E. coli, yrbF is preceded by two genes, queA and tgt, which are required for the biosynthesis of the deazaguanine derivative queuosine (Fig. 1, A and B; Ref. 32).
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The SecDF Protein-- To show that the secDF gene encodes only one protein of approximately 82 kDa, the 3' end of the secDF gene was extended with 11 codons, specifying the human c-Myc epitope (EQKLISEEDLN; Ref. 35). Next, the myc-tagged secDF gene (secDF-myc) was placed under the transcriptional control of the xylose-inducible xylA promoter and, subsequently, integrated via a double crossover replacement recombination into the amyE locus of B. subtilis, using the pX system developed by Kim et al. (36). The resulting strain was named B. subtilis XDF-Myc. As shown by Western blotting and immunodetection with c-Myc-specific monoclonal antibodies, the SecDF-Myc protein was produced in B. subtilis XDF-Myc cells growing in TY medium with 1% xylose but not in cells growing in TY medium lacking xylose. Similar results were obtained if samples for Western blotting were prepared from intact cells or protoplasts of B. subtilis XDF-Myc (Fig. 2A; only the results for protoplasts are shown). Immunodetection with SecDF-specific antibodies showed that the SecDF-Myc protein was highly overproduced in xylose-induced cells of B. subtilis XDF-Myc, as neither wild-type SecDF nor SecDF-Myc were detectable in uninduced cells (not shown). Judged from its mobility on SDS-PAGE, SecDF-Myc is a protein of about 82 kDa, which is in good agreement with the sequence-based prediction.
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Membrane Topology of SecDF-- Algorithms of Sipos and von Heijne (37) predict that the SecDF (B. subtilis) protein has 12 membrane-spanning domains, the amino and carboxyl termini being localized in the cytoplasm. Two large extracellular loops are localized between the first and second and the seventh and eighth membrane-spanning domains, respectively (Fig. 3). These predictions are in good agreement with the topology models proposed for SecD and SecF of E. coli, in which both SecD and SecF have six membrane-spanning domains with large periplasmic loops located between the first and second membrane-spanning domains (31). To verify the predicted cytoplasmic localization of the carboxyl terminus of SecDF, we studied the protease accessibility of SecDF-Myc in protoplasts. As shown by Western blotting, two trypsin-resistant SecDF-Myc-derived fragments of about 54 and 23 kDa were detectable upon incubation of intact protoplasts of xylose-induced B. subtilis XDF-Myc cells with trypsin (Fig. 2A). Under the same conditions, the B. subtilis signal peptidase SipS, which is exposed to the external side of the membrane (38), was completely degraded by trypsin (Fig. 2B), whereas the cytoplasmic protein GroEL remained unaffected (Fig. 2C). In contrast, both SecDF-Myc-derived fragments and GroEL were completely degraded by trypsin when protoplasts were lysed with 1% Triton X-100. Taken together, these findings show that the carboxyl terminus of SecDF-Myc is protected against trypsin in intact protoplasts, suggesting that the carboxyl terminus of SecDF (B. subtilis) is localized in the cytoplasm.
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Cold-sensitive Growth of B. subtilis secDF Mutants--
To analyze
the effects of SecDF depletion on growth and protein secretion, two
mutant B. subtilis strains were constructed with the
integrative plasmid pMutin2. In the first strain, denoted B. subtilis MID, the coding sequence of the secDF gene was
left intact, but the secDF promoter was replaced with the
IPTG-inducible Pspac promoter, present on pMutin2; in the
second strain, denoted B. subtilis MIF, the coding sequence
of the secDF gene was disrupted with pMutin2 (Fig.
4, A and B,
respectively). The point of truncation of the SecDF protein of B. subtilis MIF is indicated in Figs. 1 and 3. Irrespective of the
growth medium used or the presence of IPTG, both B. subtilis
MID and MIF showed growth rates at 37 °C similar to that of the
parental strain B. subtilis 168, demonstrating that under
these conditions SecDF was not essential for growth and viability of
the cells. By contrast, SecDF was important for growth in TY medium at
15 °C; compared with the parental strain (Fig. 4C, ),
the growth of B. subtilis MID (in the absence of IPTG) and
B. subtilis MIF was significantly reduced. In fact, the
growth rates of the two latter strains were reduced to the same extent
(Fig. 4C,
and
respectively), and in addition, the
cells of both strains showed a filamentous morphology (not shown).
Growth of B. subtilis MID at 15 °C could be restored by the addition of IPTG to the medium (Fig. 4C,
), although
not completely to wild-type levels. Similarly, growth of B. subtilis MIF at 15 °C could be restored to a similar level as
that of B. subtilis MID in the presence of IPTG by
introducing the secDF-myc gene in the amyE locus
(not shown), indicating that the c-Myc tag did not interfere with SecDF
function. Interestingly, the growth defects of B. subtilis
MID (in the absence of IPTG) and MIF were not observed instantaneously
upon incubation at 15 °C, as both strains showed growth rates
comparable to those of the parental strain until the mid-exponential
growth phase (A600
0.3-0.4; Fig.
4C).
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SecDF Is Required for Efficient Secretion of AmyQ-- To investigate the importance of SecDF for protein secretion at moderate levels (about 30 mg of protein per liter), the secretion of the neutral protease NprE by B. subtilis MIF was analyzed by Western blotting. Interestingly, both at 37 and 15 °C, the absence of SecDF did not result in the accumulation of pre-NprE, and similar amounts of mature NprE were secreted by B. subtilis MIF and the parental strain (not shown). To evaluate the importance of SecDF under conditions of hypersecretion, the secretion of AmyQ into the growth medium was investigated by Western blotting experiments. The results showed that B. subtilis MIF (pKTH10) secreted reduced levels of AmyQ into the medium. This was most clearly observed with cells that had been washed and resuspended in fresh medium. If the washed cells were incubated for 1 h at 37 °C, the medium of B. subtilis MIF contained about 65 ± 10% of the amount of AmyQ secreted by the parental strain (Fig. 5A). An even more drastic effect was observed at 15 °C; after 16 h of incubation, the medium of B. subtilis MIF contained about 40 ± 10% of the amount of AmyQ secreted by the parental strain (Fig. 5B). The reduced secretion of AmyQ into the medium by B. subtilis MIF was paralleled by an increased accumulation of pre-AmyQ in the cells (Fig. 5C). Since the cellular levels of mature AmyQ were not affected in the absence of intact SecDF, these data suggest that SecDF is required for the efficient translocation of pre-AmyQ but not the release of mature AmyQ from the membrane.
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Growth Phase- and Medium-dependent Transcription of the
secDF Gene--
To test whether the transcription of the
secDF gene depends on the growth phase or medium
composition, as previously shown for the signal peptidase-encoding
genes sipS and sipT (30, 41), we made use of the
transcriptional secDF-lacZ gene fusions present in B. subtilis MID and MIF (Fig. 4, A and B). Only
the results for B. subtilis MIF are documented, as similar
results were obtained with B. subtilis MID. B. subtilis MIF was grown in minimal medium, TY, or TY with 1%
glucose, and samples withdrawn at hourly intervals were assayed for
-galactosidase activity. Nearly constant levels of
-galactosidase
activity were observed during growth in minimal medium, suggesting that
the secDF gene was expressed constitutively (Fig.
8,
). In contrast, cells grown in TY
medium showed increasing levels of
-galactosidase activity during
exponential growth with a maximum at the beginning of post-exponential
growth. The
-galactosidase activity decreased in the
post-exponential growth phase (Fig. 8,
), suggesting that
secDF promoter activity was highest during the transition
from exponential to post-exponential growth. Interestingly, the
addition of 1% glucose to TY medium caused a drastic increase in the
-galactosidase levels of cells in the post-exponential growth phase,
showing that glucose strongly stimulates the transcription of the
secDF gene (Fig. 8,
). Thus, the transcription of the secDF gene depends on the growth phase and growth medium.
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DISCUSSION |
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In the present study, we demonstrate that the SecDF protein of B. subtilis is required for efficient translocation and processing of the secretory precursor pre-AmyQ and the secretion of mature AmyQ into the growth medium. The reduced secretion of AmyQ by cells lacking intact SecDF was paralleled by the accumulation of pre-AmyQ. These findings show that SecDF (B. subtilis), like SecD and SecF of E. coli, is required for protein translocation across the cytoplasmic membrane and that the function of SecDF in protein translocation is most likely conserved among eubacteria. Notably, the SecDF-depleted cells did not accumulate mature AmyQ. Thus, it seems that SecDF (B. subtilis), unlike SecD of E. coli (16, 34), is not required for the release of mature proteins from the membrane.
The observation that secDF mutants grow at reduced rates at low temperature indicates that protein translocation in B. subtilis is intrinsically cold-sensitive, as previously suggested for protein translocation in E. coli (42). However, in contrast to E. coli mutants with disrupted secD and/or secF genes, which are cold-sensitive for growth and barely viable at 37 °C (43), B. subtilis strains, which contain a disrupted secDF gene (this paper) or which completely lack the secDF gene (not shown), show normal growth and cell viability at 37 °C and do not stop growing at low temperature. SecDF was only essential for growth at 15 °C when AmyQ was overproduced. These findings indicate that SecDF is not strictly required for protein translocation in B. subtilis and that the degree in which SecDF is required depends on the level of synthesis of secretory proteins. The latter view is supported by the observation that the secretion of NprE, which was produced at about 30-50-fold lower levels than AmyQ, was not affected in strains lacking SecDF, even at low temperature (not shown). In addition, even when AmyQ was overproduced, SecDF-depleted cells did not stop to grow instantaneously after a shift from 37 to 15 °C, as growth defects were only observed after cells had entered the mid-exponential growth phase. The latter observation suggests that SecDF is not required for early exponential growth, which is consistent with the fact that exponentially growing cells of B. subtilis secrete only few proteins (see Ref. 44). Although SecDF is involved in protein secretion, which is a post-exponential growth phase-specific phenomenon in B. subtilis, this protein is neither required for the development of competence for DNA binding and uptake nor sporulation (not shown), two post-exponential processes that require the activity of SecA (22).
We have previously shown that the transcription of two signal peptidase-encoding genes, sipS and sipT, is concerted with that of the genes for most secretory proteins, which is temporally controlled, being high in the post-exponential growth phase (30, 41). Our present data show that the transcription of secDF is regulated differently as follows: 1) when cells were grown in minimal medium, secDF was transcribed constitutively, whereas the transcription of sipS and sipT was temporally controlled; 2) when cells were grown in TY medium, secDF transcription was maximal in the early post-exponential growth phase, whereas the levels of sipS and sipT transcription that were low in the exponential growth phase started to increase in the transition phase and remained high in the post-exponential growth phase; and 3) when cells were grown in TY medium with 1% glucose, secDF transcription was highly stimulated in the post-exponential growth phase, whereas sipS transcription was not stimulated.2 The effect of glucose on the transcription of secDF is remarkable, because the transcription of most genes for secretory proteins is repressed by glucose (45) and because glucose did not significantly stimulate the transcription of genes for other components of the secretion machinery, such as SecA and the type II signal peptidase.2 Presently, it is difficult to explain why the patterns of secDF transcription do not correlate with those of genes specifying secretory proteins, or the signal peptidases SipS and SipT. One possible explanation is that the turnover rates of SecDF depend on the growth conditions and that B. subtilis can maintain a sufficient level of the SecDF protein through controlled transcription of the secDF gene.
In contrast to most other organisms, the SecD and SecF equivalents of B. subtilis 168 are jointly present in one polypeptide, which can thus be considered as a "molecular siamese twin." This observation suggests that, in general, SecD and SecF proteins have a head-to-tail orientation in the translocase complex. The presence of one SecDF protein instead of separate SecD and SecF proteins is probably not a peculiarity of B. subtilis 168. Preliminary sequence data suggest that at least two other organisms, Chlamydia trachomatis and Deinococcus radiodurans, also contain genes specifying SecDF-like proteins.3 As a consequence of the fusion between the SecD and SecF domains, SecDF (B. subtilis) seems to have 12 transmembrane regions, the amino- and carboxyl termini being localized in the cytoplasm. Thus, SecDF (B. subtilis) shows structural similarity to a large group of secondary solute transporters for which the presence of 12 membrane-spanning domains is characteristic (46). As SecDF (B. subtilis) also shows sequence similarity to certain solute transporters (i.e. AcrF and ActII-3), our findings suggest that SecDF (B. subtilis) represents a novel type of the SecD and SecF proteins, with structural resemblance to secondary solute transporters.
Comparison of SecDF (B. subtilis) with SecD and SecF proteins from various organisms revealed 10 patterns of conserved residues. Our results show that at least one of the three conserved regions, F2, F3, and F4, is critical for SecDF function, as F2 is disrupted and F3 and F4 are absent from the truncated SecDF protein of B. subtilis MIF. It is presently not known to what extent the other conserved regions are required for SecDF function.
Finally, our observation that secretion defects in B. subtilis strains lacking SecDF are only evident under conditions of hypersecretion shows that SecDF is required to maintain a high capacity for protein secretion. Thus, at least three mechanisms for SecDF function in B. subtilis are conceivable as follows: first, SecDF might stimulate the assembly of active pre-protein translocase complexes; second, SecDF might stimulate PMF-driven protein translocation; and third, SecDF activity might be required to clear the translocation channels from prematurely folded pre-proteins or signal peptides, which might jam the channel or inhibit SecA under conditions of high level production of secretory proteins. The latter concept would be consistent with the observation that SecDF shows structural similarity to secondary solute transporters.
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ACKNOWLEDGEMENTS |
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We thank Dr. M. Sarvas for sera against
B. amyloliquefaciens -amylase; Drs. J. Swaving and
A. J. M. Driessen for sera against SecDF (B. subtilis); Drs. L. de Leij and W. Helfrich for c-Myc-specific monoclonal antibodies; Dr. V. Vagner for plasmid pMutin2; Drs. T. Wiegert and W. Schumann for plasmids pKTH10-BT and pX; and Drs. H. Tjalsma, J. Jongbloed, and R. Freudl for stimulating discussions. We
are indebted to Dr. S. D. Ehrlich for continuous support.
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FOOTNOTES |
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* 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.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) AF024506.
b Supported by European Union(EU) Biotechnology Grant Bio2-CT93-0254.
d Supported by European Union Biotechnology Grants Bio2-CT93-0254 and Bio4-CT96-0097.
f Supported by European Union Biotechnology Grant Bio2-CT93-0272.
g Supported by the Dutch Ministry of Economic Affairs through Associatie Biologische Onderzoeksscholen Nederland.
i To whom correspondence should be addressed. Tel.: 31503632107; Fax: 31503632348; E-mail: j.m.van.dijl{at}biol.rug.nl.
The abbreviations used are:
PMF, proton motive
force; IPTG, isopropyl--D-thiogalactopyranosidePCR, polymerase chain reactionTY, tryptone/yeast extractPAGE, polyacrylamide gel electrophoresis.
2 A. Bolhuis, C. P. Broekhuizen, A. Sorokin, M. L. van Roosmalen, G. Venema, S. Bron, W. J. Quax, and J. Maarten van Dijl, unpublished observations.
3 Accessible through chlamydia-www.berkeley.edu:4231 and www.tigr.org/tdb/mdb/mdb.html.
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REFERENCES |
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