AmyA, an {alpha}-Amylase with {beta}-Cyclodextrin-Forming Activity, and AmyB from the Thermoalkaliphilic Organism Anaerobranca gottschalkii: Two {alpha}-Amylases Adapted to Their Different Cellular Localizations

Two ${alpha}$ -amylase genes from the thermophilic alkaliphile Anaerobrancagottschalkii were cloned, and the corresponding enzymes, AmyAand AmyB, were investigated after purification of the recombinantproteins. Based on their amino acid sequences, AmyA is proposedto be a lipoprotein with extracellular localization and thusis exposed to the alkaline milieu, while AmyB apparently representsa cytoplasmic enzyme. The amino acid sequences of both enzymesbear high similarity to those of GHF13 proteins. The differentcellular localizations of AmyA and AmyB are reflected in theirphysicochemical properties. The alkaline pH optimum (pH 8),as well as the broad pH range, of AmyA activity (more than 50%activity between pH 6 and pH 9.5) mirrors the conditions thatare encountered by an extracellular enzyme exposed to the mediumof A. gottschalkii, which grows between pH 6 and pH 10.5. AmyB,on the other hand, has a narrow pH range with a slightly acidicpH optimum at 6 to 6.5, which is presumably close to the pHin the cytoplasm. Also, the intracellular AmyB is less tolerantof high temperatures than the extracellular AmyA. While AmyAhas a half-life of 48 h at 70°C, AmyB has a half-life ofonly about 10 min at that temperature, perhaps due to the lackof stabilizing constituents of the cytoplasm. AmyA and AmyBwere very similar with respect to their substrate specificityprofiles, clearly preferring amylose over amylopectin, pullulan,and glycogen. Both enzymes also hydrolyzed ${alpha}$ -, ß-,and ${gamma}$ -cyclodextrin. Very interestingly, AmyA, but not AmyB, displayedhigh transglycosylation activity on maltooligosaccharides andalso had significant ß-cyclodextrin glycosyltransferase(CGTase) activity. CGTase activity has not been reported fortypical ${alpha}$ -amylases before. The mechanism of cyclodextrin formationby AmyA is unknown.

INTRODUCTION

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Introduction

Few anaerobic bacteria are able to grow at a combination ofelevated temperature and alkaline pH, two factors which putconsiderable stress on the cells. Species known to grow optimallyat pH 8.5 and 55°C or higher belong to the low-G+C gram-positivebacteria (4, 29), with the exception of "Thermopallium natronophilum"(proposed name). To our knowledge, they are Anaerobranca horikoshii,Anaerobranca gottschalkii, Anaerobranca californiensis, Clostridiumparadoxum, Thermosyntropha lipolytica, and Desulfotomaculumalkaliphilum (5, 6, 13, 20, 21, 22).

Surprisingly, a number of enzymes isolated from mesophilic organismsare known to exhibit a combination of high thermostability andalkali tolerance. Several ${alpha}$ -amylases, mostly from Bacillus species,have been described as displaying these rare properties (3,14, 17). Such ${alpha}$ -amylases and other saccharolytic enzymes in generalare of considerable commercial interest for industrial processes,e.g., in the paper industry and in starch processing. Also,enzymes with these properties are of importance as additivesto laundry and dishwashing detergents. Despite the potentialof thermoalkaliphilic microorganisms as sources of biotechnologicallyinteresting biocatalysts, very few of their enzymes have beencharacterized to date, among them an alkalitolerant and thermostabletype I pullulanase and a ß-cyclodextrin glycosyltransferase(CGTase) from A. gottschalkii (2, 23).

Gram-positve A. gottschalkii was isolated from humid soil ata hot inlet of an alkaline soda lake, Lake Bogoria, Kenya. Theanaerobic organism grows in a range of pH 6.0 to 10.5 and 30to 65°C with the optimum at pH 9.5 and 50 to 55°C anda supplementation of 230 mM Na⁺ ions. It is reported to growheterotrophically on various mono- and polysaccharides and polypetides(21).

Microorganisms that live in an alkaline environment have tocope with a substantial pH gradient across the cytoplasm membrane.The pH conditions for extra- and intracellular enzymes differgreatly. In consequence, in an alkaline environment, the differencesbetween the biochemical optimum conditions of extracellularand intracellular enzymes can be expected to be much greaterthan in neutrophiles, where the pH values outside and insidethe cells are similar. The amylases of the neutrophile Thermoactinomycesvulgaris, for example, differ in their cellular localizations,but their amino acid sequences and physicochemical characteristicsare similar (25).

In this communication, we report the heterologous expression,purification, and comparison of the biochemical characteristicsof two ${alpha}$ -amylases with different cellular localizations fromthe thermoalkaliphilic bacterium A. gottschalkii.

MATERIALS AND METHODS

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Materials and Methods

Sequence analysis.
Protein sequence databases were searched with the BLAST algorithmavailable at the National Center for Biotechnology Informationserver (http://www.ncbi.nlm.nih.gov) (1). Lipoprotein signalsequence prediction was carried out using the LipoP 1.0 serverof the Center for Biological Sequence Analysis, Technical Universityof Denmark (http://www.cbs.dtu.dk) (9).

Anaerobranca gottschalkii culture conditions.
Anaerobranca gottschalkii DSM 13577 was grown anaerobicallyas previously described (21) at 50°C with 0.5% starch asa carbon source. The supernatant of a 100-liter fermentor culturewas concentrated to 57 ml by cross-flow filtration using a 30-kDamembrane (Filtron, Karlstein, Germany).

Construction of AmyA and AmyB expression clones.
The genes coding for AmyA and AmyB were amplified from a genomiclibrary of A. gottschalkii (Epidauros, Bernried, Germany) (11).While for amyB the full-length sequence of the open readingframe (ORF) was obtained, the amyA gene was amplified withoutits putative signal peptide-encoding sequence. A new start codonwas introduced. The primer sequences for amyA were 5'-GAA TTCATG ACC AGT GAT AAG CAA GGT CCC CAA GAG ACC-3' (fwd; the EcoRIsite is underlined) and 5'-AAG AGC TCA ATT TTT AAG ACA AAT AGAAAA GGA AGA AGA ATT-3' (rev), and those for amyB were 5'-ATTAGG ATT CAT ATG CAA CAA GAG ATT TTA TAT TTT-3' (fwd; the NdeIsite is underlined) and 5'-C AGA AAA AAG CTT TTT ATT TTT CAGGGG C-3' (rev; the HindIII site is underlined). The amplifiedproducts were initially cloned into pTOPO (Invitrogen, Karlsruhe,Germany) and pBluescript (Stratagene, Heidelberg, Germany) vectors,respectively, before being recloned into pET21c overexpressionvectors (Novagen, Schwalbach, Germany). The correct cloningof both amylase ORFs was confirmed by sequencing and restrictionenzyme analyses. All recombinant techniques were performed inEscherichia coli XL1-blue, E. coli DH5 ${alpha}$ , and E. coli BL21.

Expression and crude-extract preparation of the recombinant ${alpha}$ -amylases.
Liquid cultures (two, 1 liter each) of the recombinant E. coliclones carrying the pET21c-amyA construct and the pET21c-amyBconstruct were grown in 5-liter baffle flasks overnight at 37°Cin Luria-Bertani medium (1% [wt/vol] tryptone, 0.5% [wt/vol]yeast extract, 0.5% [wt/vol] NaCl) supplemented with 50 µgml^–1 ampicillin. When the optical densities (600 nm) ofthe cultures reached approximately 0.6, the T7 promoter of thepET vectors was induced with 1 mM isopropyl-1-thio-ß-D-galactoside(IPTG), and incubation was continued overnight. Cells were harvestedby centrifugation (10,400 x g; 15 min; 4°C), washed, andresuspended in 30 ml phosphate-buffered saline (pH 8.5) in thecase of the AmyA-expressing culture or 20 ml 20 mM Tris-HCl(pH 8.0) in the case of the AmyB-expressing culture. The cellswere disrupted by twofold passage through a French pressurecell (American Instruments, Silver Springs, MD). After separationfrom the cell debris by centrifugation (20,000 x g; 30 min;4°C), the supernatants were incubated at 65°C for 20min in order to denature the thermolabile host proteins, whichwere sedimented at 20,000 x g for 15 min at 4°C.

Purification of AmyA.
The cleared supernatant from the heat-treated crude extractof E. coli BL21(pET21c-amyA) containing $~$ 95 mg protein was dialyzedagainst 20 mM Tris-HCl (pH 8.0) buffer and subjected to anion-exchangechromatography on a Source 15Q XK 26/10 column (Amersham Biosciences,Freiburg, Germany) equilibrated with the same buffer. Elutionwas done with a two-step gradient (0 to 0.4 M NaCl in 10 columnvolumes [CV]; 0.4 to 1 M NaCl in 1 CV) in the same buffer ata flow rate of 10 ml min^–1. Amylase activity-containingfractions, which eluted at about 0.3 M NaCl, were pooled anddialyzed against 20 mM Tris-HCl (pH 8.0) buffer. In order tofurther purify the protein by hydrophobic interaction chromatography,the pool ( $~$ 32 mg protein) was adjusted to 5 M NaCl and appliedto a phenyl-Sepharose HP XK 16/10 column (Amersham Biosciences)equilibrated with 20 mM Tris-HCl (pH 8.0) buffer containing5 M NaCl. Elution was performed with a two-step gradient (5to 3 M NaCl in 1 CV; 3 to 0 M NaCl in 9 CV) in 20 mM Tris-HCl(pH 8.0) buffer at a flow rate of 2 ml min^–1. AmyA-containingfractions, which eluted at $~$ 0.5 M NaCl, were pooled and dialyzedagainst 20 mM Tris-HCl (pH 8.0). The purity of the resultingenzyme preparation was >95%, as confirmed by sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE).

Purification of AmyB.
The cleared supernatant from the heat-treated crude extractof E. coli BL21(pET21c-amyB), about 165 mg protein, was dialyzedagainst 20 mM Tris-HCl (pH 8.0) buffer and applied to a Source15Q XK 26/10 column (Amersham Biosciences) equilibrated withthe same buffer. Elution was done with a two-step gradient (0to 0.4 M NaCl in 10 CV; 0.4 to 1 M NaCl in 2 CV) in the samebuffer at a flow rate of 5 ml min^–1. AmyB-containing fractionswere pooled and dialyzed against 20 mM Tris-HCl (pH 8.0) buffer.The purity of the resulting enzyme preparation was >95%,as confirmed by SDS-PAGE.

Analytical size exclusion chromatography.
In order to determine the native molecular masses of the purifiedproteins, analytical size exclusion chromatography was carriedout using a Superdex 200 prep grade HiLoad 16/60 column (AmershamBiosciences). An isocratic gradient of 20 mM Tris-HCl (pH 8.0)with the addition of 150 mM NaCl was applied.

Gel electrophoresis.
SDS-PAGE according to the method of Laemmli (12) was routinelyperformed to test the purity of the samples during purificationand to estimate the molecular masses of proteins under denaturingconditions. SDS-PAGE was carried out with gels containing 12%(vol/vol) acrylamidebisacrylamide in Mini-Protean II electrophoresisunits (Bio-Rad, Munich, Germany), and the gels were stainedwith Coomassie brilliant blue. Sizes of the analyzed proteinswere estimated by comparison with the standard protein markermixture SDS-6H (Sigma-Aldrich, Taufkirchen, Germany) separatedon the same gel.

For activity staining, the SDS-PAGE gel was equilibrated in0.2 M phosphate buffer (pH 7.0) for 45 min, followed by an overnightincubation in 0.2 M phosphate buffer containing 1% soluble starch.Amylase activity was determined by incubating the gel in thisbuffer at 75°C for 15 min. The remaining starch was stainedwith Lugol solution (0.3% [wt/vol] I₂, 0.6% [wt/vol] KI), aprocess that left clear halos around sites of amylolytic activity.

Activity assay.
A 3,5-dinitrosalicylic acid-based method for measuring the enzymaticrelease of reducing groups from starch was used as a standardtest (19). The reaction mixture contained 250 µl substrate(0.5% [wt/vol] soluble starch [Sigma-Aldrich] or other polysaccharidesas specified in the text); 100 µl 200 mM McIlvaine bufferadjusted to pH 8.0 for AmyA and pH 6.0 for AmyB, respectively;150-x µl distilled H₂O; and x µl appropriately dilutedenzyme (where x represents the volume of enzyme preparation).After incubation for 20 min at 60°C for AmyA and 15 minat 50°C for AmyB, 750 µl of 3,5-dinitrosalicylic acidsolution (1% [wt/vol] 3,5-dinitrosalicylic acid, 0.2% [vol/vol]phenol, 0.05% [wt/vol] Na₂SO₄, 20% KNa-tartrate, 1% [wt/vol]NaOH in H₂O_bidest) was added, and the mixture was incubatedfor 15 min at 98°C. Absorption was measured at 575 nm, andthe specific activity was calculated using maltose as a standard.One unit of ${alpha}$ -amylase is defined as the amount of enzyme thatliberates 1 µmol of reducing groups per min.

Influences of pH and temperature on activity.
The influence of pH on AmyA was measured at 60°C and onAmyB at 50°C with McIlvaine buffer adjusted to various pHvalues, using the standard assay described above. The influenceof temperature on the enzyme activity was determined using standardassay reactions incubated at temperatures ranging from 35 to80°C.

Thermoinactivation.
The enzymes were diluted to a protein concentration of about50 µg ml^–1 in McIlvaine buffer adjusted to pH 8.0(AmyA) or pH 6.0 (AmyB) at selected temperatures. The kineticsof thermoinactivation of the recombinant enzymes was determinedthrough preincubation of the diluted enzyme at various temperaturesfor different intervals of time, followed by determination ofresidual activity with the standard enzyme assay.

Influence of metal ions.
The effect of metal ions was analyzed at 1 mM final concentrationsof a variety of mono- and divalent cations in a HEPES (pH 8.0)and a 2-morpholinoethanesulfonic acid (MES) (pH 6.0) buffersystem for AmyA and AmyB, respectively, in order to avoid precipitationof some of the ions with the McIlvaine buffer components.

The effect of EDTA on AmyA activity was analyzed in HEPES, McIlvaine,and Tris buffers, all at 50 mM at pH 8.0. The enzyme was dilutedto 50 µg ml^–1 with buffer and incubated with 5 mMEDTA for 1 h prior to the determination of activity in the samebuffer system.

Analysis of sugars by TLC.
Thin-layer chromatography (TLC) of mono- and oligosaccharideswas done on 0.2 mm silica gel-coated aluminum sheets (Type 60;Merck, Darmstadt, Germany) with a solvent system containing1-propanol-ethyl acetate-H₂O at a volume ratio of 6:1:3 or 1-propanol-nitromethane-H₂Oat a volume ratio of 5:3:2. The chromatograms were sprayed withanilinediphenylamine reagent (1% [wt/vol] diphenylamine, 1%[vol/vol] aniline in acetone mixed with 0.1 volume 87% [vol/vol]phosphoric acid prior to use) and baked for 10 min at 160°Cto visualize the carbohydrate spots.

ß-Cyclodextrin assay.
The presence of cylodextrins was determined using a phenolphthaleincolorimetric assay (27). After incubation for 1 h at 60°C,a standard reaction mixture aliquot of 100 µl was addedto 2 ml phenolphthalein test solution ready mixed from 10 mlNa₂CO₃ (0.2 M) and 17 µl of phenolphthalein stock solution(1% [wt/vol] phenolphthalein in 50% [vol/vol] ethanol). Absorptionwas measured at 537 nm against a blank of 100 µl maltooligosaccharidemixture (0.1% [wt/vol]) and 2 ml phenolphthalein test solution.The concentration of ß-cyclodextrin was calculatedby comparison with assay results obtained with defined amountsof ß-cyclodextrin standard.

RESULTS

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Results

Sequence analysis and enzyme localization.
The amyA gene (gb:AY842299) from A. gottschalkii has a sizeof 1,599 bp and codes for a 532-amino-acid polypeptide. A lipoproteinsignal peptide of 21 residues was found by using the LipoP 1.0prediction program for lipoproteins, which uses a hidden Markovmodel to distinguish between lipoproteins (SPase II-cleavedproteins), SPase I-cleaved proteins, cytoplasmic proteins, andtransmembrane proteins. The potential cleavage site in the sequenceMTSKILRVLLVFLLIFAIVG-CTS(...) is predicted between glycine 20and cysteine 21. In order to avoid expression problems, amyAwas cloned without the signal peptide-encoding sequence, andcysteine 21 was mutated to a methionine. The resulting ORF onthe pET21-amyA vector had a length of 1,539 bp and coded fora protein of 512 amino acids.

The amino acid sequence of AmyA shows between 42 and 45% identitywith a putatively exported ${alpha}$ -amylase from Bacillus megaterium(gb:P20845) (18), a neopullulanase from Paenibacillus sp. strainKCTC8848P (gb:AAL07400) (10), and ${alpha}$ -amylase 3 from Dictyoglomusthermophilum, another putative extracellular protein (gb:P14899)(8), which constitute the three best-scored hits with the BLASTalgorithm.

No indications of a signal peptide could be found in the 443-residuepolypeptide that is encoded by the 1,331-bp amyB ORF (gb:AY842298),indicating that AmyB presumably is a cytoplasmic protein. TheAmyB amino acid sequence shows 43% identity with that of the ${alpha}$ -amylase from Thermoactinomyces vulgaris (gb:CAA49465) (7),39% identity with a ß-/ ${alpha}$ -amylase precursor from Bacilluspolymyxa (gb:A29130) (26), and 34% identity with a putativeglycoside hydrolase from Deinococcus radiodurans (gb:AAF11034)(28). Altogether, the amino acid sequences of both AmyA andAmyB bear high similarity to glycoside hydrolase family 13 (GHF13)proteins; the four highly conserved motifs typical of GHF13enzymes were found in both A. gottschalkii ${alpha}$ -amylases (Table1). Beyond the conserved regions, the two studied proteins hadan overall sequence identity of 33%.

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TABLE 1. Comparison of the four highly conserved ${alpha}$ -amylase regions of AmyA and AmyB from A. gottschalkii with TAKA-amylase from Aspergillus oryzae (gb:0901305A) (24)^a

The presumed localizations of AmyA and AmyB in the culture supernatantand the cytosolic fraction of an A. gottschalkii culture werevalidated by SDS-PAGE and subsequent activity staining. Themobilities of the bands with amylolytic activity correspondedwell with the expected sizes of the enzymes. Obviously, at leastpart of putative lipoprotein AmyA is released into the culturesupernatant (Fig. 1).

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FIG. 1. SDS-PAGE analysis and activity staining of A. gottschalkii culture supernatant (A) and cytosolic crude extract (B). Lanes S, size standard; lane 1, Coomassie-stained culture supernatant; lane 2, activity-stained culture supernatant; lane 3, Coomassie-stained cytosolic crude extract; lane 4, activity-stained cytosolic crude extract.

Purification.
After induction with 1 mM IPTG, the overnight flask culturesof E. coli BL21 cells transformed with pET21c-amyA yielded approximately1.6 g cells liter^–1. Following the disruption of the E.coli cells, recombinant AmyA was initially concentrated by heattreatment at 65°C for 20 min, which resulted in denaturationof the majority of the host proteins. After two subsequent chromatographicseparation steps, i.e., anion-exchange followed by a hydrophobicinteraction chromatography, an enzyme preparation appearingas a single band in SDS-PAGE was obtained. AmyB was purifiedthrough heat treatment of the crude extract, followed by anion-exchangechromatography, leading to a homogenous enzyme preparation asjudged by SDS-PAGE (data not shown). With starch as the substrate,the specific activities were 52 U/mg for purified AmyA and 220U/mg for purified AmyB.

The apparent sizes of the proteins according to SDS-PAGE arein agreement with the molecular masses derived from the aminoacid sequences. The conceptual translation masses of the full-lengthopen reading frames of the amyA (as cloned without the signalpeptide-encoding sequence) and amyB genes are 59,146 Da and51,702 Da, respectively. Recombinant AmyB had a molecular massof 108 kDa as determined by its elution behavior during gelfiltration chromatography, which suggests the active moleculeexists as a dimer. For AmyA, a molecular mass of 58 kDa wasdetermined, which points to a monomer as the active quaternaryform.

Biochemical characterization and substrate specificity.
With a 20-min assay using starch as the substrate, the maximumenzymatic activity of AmyA was measured at 70°C and pH 8.0.For AmyB, maximum activity was found at 55°C and pH 6.0(Fig. 2). The half-life of AmyA at 70°C was 48 h. At 60°C,no significant loss of activity was found even after 60 h ofpreincubation. AmyB retained more than 80% activity after 5h of preincubation at 50°C. At 65°C, the maximum growthtemperature of A. gottschalkii (21), AmyB had a half-life of60 min (Fig. 3).

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FIG. 2. Effects of temperature (A) and pH (B) on the activities of AmyA (white squares) and AmyB (black squares). All measurements were carried out in McIlvaine buffer calibrated at the respective pH and temperature.

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FIG. 3. Effects of long-term incubation at elevated temperatures on AmyA (A) and AmyB (B). AmyA was incubated at 60°C (black circles), 70°C (black inverted triangles), and 75°C (white squares). AmyB was incubated at 50°C (white circles), 60°C (black circles), 65°C (white triangles), and 70°C (black inverted triangles).

AmyA and AmyB were hydrolytically active on a variety of ${alpha}$ -1,4-linkedcarbohydrates, with amylose being the best substrate in bothcases (Table 2). The main products of AmyA hydrolysis were maltoseand glucose, except with pullulan as a substrate. Substratesexclusively containing non- ${alpha}$ -1,4-glycosidic bonds, such as mannan,dextran, and cellulose, were not degraded. AmyB action resultedin glucose, maltose, and maltotriose as final products, withmaltose being the major product. Both enzymes hydrolyzed amylosewith an endomechanism, which was determined by thin-layer chromatographywith samples drawn at different time points during amylose degradation.First, maltooligosaccharides of various lengths were generated,and later, glucose and maltose or glucose, maltose, and maltotriosewere accumulated as final products (data not shown). On thebasis of their substrate specificities and characteristics ofproduct formation by cleavage of ${alpha}$ -1,4-glycosidic bonds in polysaccharides,the A. gottschalkii enzymes AmyA and AmyB were classified as ${alpha}$ -amylases (EC 3.2.1.1).

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TABLE 2. Substrate specificities of the recombinant ${alpha}$ -amylases

With short maltodextrins as substrates, AmyA displayed significanttransferase activity, as well as hydrolysis (Fig. 4). Strikingly,in addition to linear maltodextrins, a small amount of cyclodextrinwas formed, which was identified as ß-cyclodextrinby its mobility in TLC analysis and its complexation propertyin a colorimetric assay with phenolphthalein. In a standardassay with 23.5 µg ml^–1 AmyA, about 1.6% of theinitial 25 mM maltotriose was converted to ß-cyclodextrinwith a specific activity of 0.3 U/mg. Over time, the maltodextrinsformed, as well as the ß-cyclodextrin, were degradedagain by the enzyme. For AmyB, no significant transferase activityor cyclodextrin formation was observed.

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FIG. 4. TLC analysis of product formation from various maltodextrins by AmyA. Maltodextrins (25 mM) were digested with recombinant AmyA at 24 µg/ml in McIlvaine buffer for 1 h at 60°C. The products were separated on a silica gel TLC plate in 1-propanol-ethyl acetate-H₂O (6:1:3) (vol/vol/vol). Lane S, G1-G7 oligosaccharide standard; lane 1, maltose; lane 2, maltose after incubation with AmyA; lane 3, maltotriose; lane 4, maltotriose after incubation with AmyA; lane 5, maltotetraose; lane 6, maltotetraose after incubation with AmyA; lane 7, maltopentaose; lane 8, maltopentaose after incubation with AmyA; lane 9, maltohexaose; lane 10, maltohexaose after incubation with AmyA; lane 11, maltoheptaose; lane 12, maltoheptaose after incubation with AmyA. The arrows indicate the formed ß-cyclodextrin.

Effects of metal ions and other reagents.
The effects of various metal ions added to the reaction mixturewere tested. In order to avoid precipitation, McIlvaine bufferwas replaced with HEPES (AmyA) and MES (AmyB), although AmyAdisplayed significantly lower activity in HEPES buffer thanin McIlvaine buffer. Ca²⁺, Sr²⁺, and Ba²⁺ at a concentrationof 1 mM had a positive effect on AmyA. With Ca²⁺ supplementation,its activity was increased twofold, while Sr²⁺ and Ba²⁺ hada slightly weaker effect on the enzyme. Mn²⁺ and Co²⁺ reducedAmyA activity, while Ni²⁺, Cu²⁺, Zn²⁺, and Cd²⁺ completely inhibitedthe enzyme. NaCl in concentrations above 50 mM slightly enhancedthe activity of AmyA. The most prominent effects on AmyB weregenerated by the addition of 1 mM Mn²⁺, Co²⁺, Cu²⁺, and Zn²⁺,with all of these ions strongly inhibiting the recombinant enzyme(data not shown).

The addition of ethanol (5% [vol/vol]) and 2-mercaptoethanol(2 mM) had no effect on AmyA activity, whereas glycerol (5%[vol/vol]), dithiothreitol (10 mM), and NAD (6 mM) had minorinhibitory effects on the recombinant enzyme (data not shown).

EDTA was not found to be inhibitory for AmyA in HEPES and McIlvainebuffer systems. Even after preincubation for 1 h at 60°Cwith 5 mM EDTA, the enzyme activity was not significantly reduced,indicating that Ca²⁺, although stimulating, was not requiredfor activity of the recombinant enzyme in these buffers. Curiously,when Tris buffer was used, EDTA had an inhibitory effect, whichcould be completely reversed by the addition of 10 mM Ca²⁺ (Fig.5).

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FIG. 5. Effects of EDTA on AmyA under different buffer conditions. The enzyme was diluted to 50 µg ml^–1 with the corresponding buffer and preincubated with CaCl₂ or EDTA at 60°C for 1 h. Black bars, AmyA without additive; light-gray bars, AmyA with 5 mM EDTA; white bars, AmyA with 5 mM CaCl₂; dark-gray bar, AmyA with 5 mM EDTA plus 10 mM CaCl₂ added to the activity test. The effect of CaCl₂ in MacIlvaine buffer was not determined due to precipitation.

DISCUSSION

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Discussion

The ${alpha}$ -amylases AmyA and AmyB from the anaerobic thermoalkaliphilicbacterium A. gottschalkii were heterologously overexpressedin E. coli and biochemically characterized. AmyA, a putativelipoprotein, was expressed without its signal peptide, resultingin a monomer of 59 kDa. AmyB was found to be a homodimer withtwo 52-kDa subunits. Based on their modes of hydrolytic action(endomechanism) and their substrates ( ${alpha}$ -1,4-linked polysaccharides),both enzymes were classified as ${alpha}$ -amylases. They both showedsequence similarity to members of glycoside hydrolase family13. It has been argued that the last two amino acid residuesin the conserved region II of GHF13 proteins are of criticalimportance for substrate specificity (15). Both ${alpha}$ -amylases examinedhave a lysine and a histidine in those positions, which supportsthe theory that these two residues appear in enzymes with specificityfor ${alpha}$ -1,4-glycosidic bonds.

Apparently, AmyA features, in addition to the typical ${alpha}$ -amylasehydrolytic activity, the ability to act as a 4- ${alpha}$ -glucanotransferase,a combination of activities not unusual for ${alpha}$ -amylases. However,it is noteworthy that AmyA has significant ß-cyclodextrin-formingactivity, which is unprecedented for typical ${alpha}$ -amylases. On theother hand, cyclodextrin glycosyltransferases are known to havevarious degrees of transferase activity on linear maltodextrins("disproportionation activity"), as well as hydrolytic activity,in addition to their main activity, i.e., cyclodextrin formation.Some CGTases have quite high ${alpha}$ -amylase activity, e.g., the CGTasefrom Thermoanaerobacterium thermosulfurigenes EM1 (30), whosehydrolytic activity (23 U/mg) is only about fourfold smallerthan its CGTase activity. AmyA from A. gottschalkii has broadenedthe spectrum of cyclodextrin-forming enzymes, being an enzymewith low cyclodextrin glycosyltransferase activity (0.3 U/mg)compared to its hydrolytic activity (52 U/mg). Apart from belongingto the same glycoside hydrolase family (GHF13), the primarystructure of AmyA is not similar to those of typical CGTases.It will be interesting to compare the crystal structure of AmyA,once available, with the high-resolution structures of CGTasesin order to understand how cyclodextrin formation is accomplishedby AmyA. The physiological relevance of the cyclodextrin-formingactivity of AmyA, however, is arguable, since A. gottschalkiihas an extracellular, recently characterized CGTase with a specificactivity of 210 U mg^–1 (23).

The different cellular localizations of AmyA and AmyB are reflectedin their physicochemical characteristics; in particular, thepH optima, as well as the range of pH values, of the A. gottschalkiiamylases mirror the pH conditions at the cellular locationswhere the enzymes are predicted to be found. AmyA shows activityover a broad pH range from 6.0 to 9.5, with an optimum at pH8.5. As a probable lipoprotein located outside the cell, theenzyme is exposed to the alkaline milieu of the habitat. A.gottschalkii grows between pH 6.0 and pH 10.5, a range correspondingto the pH range of the protein. Another extracellular enzymeof A. gottschalkii, a type I pullulanase (PulAg), which is alsopredicted to be a lipoprotein, is active from pH 7.0 to 9.5,with an optimum at pH 8.0 (2). This activity range coincidesvery well with that of the recombinant AmyA. The same is truefor the temperature-activity profiles of both amylolytic enzymes.Using a 20-min and a 10-min assay, respectively, at their optimalpHs, both AmyA and PulAg displayed maximum rates of substratehydrolysis at 70°C. The physicochemical characteristicsof the extracellular CGTase from A. gottschalkii differ onlyslightly from this. The enzyme shows maximum activity at pH6 to 9 and 65°C in a 45-min assay (23).

Few ${alpha}$ -amylases are active at both temperatures above 65°Cand alkaline pH values of 7.5 or higher. All of them are proteinsfrom Bacillus species, such as the ${alpha}$ -amylases from Bacillus sp.strain TS-23, with an activity optimum at pH 9.0 and 70°C;from B. megaterium, with an activity optimum at pH 8.9 and 70°C;and from Bacillus licheniformis CUMC 305, with an activity optimumat pH 9.0 and 90°C. AmyA from A. gottschalkii, a non-Bacillusorganism, is a notable exception (3, 14, 17).

AmyB, the intracellular ${alpha}$ -amylase, has an optimum at pH 6.0 anda much narrower pH range than AmyA. Since the intracellularpH of alkaliphiles is more acidic than the medium, intracellularenzymes can be expected to be somewhat less alkaliphilic thantheir extracellular counterparts. Due to cell homeostasis, changesof the internal pH are small, which allows enzymes to be lesstolerant of pH changes. In addition, the intracellular AmyBis less tolerant of high temperatures than the extracellularAmyA. While AmyA has a half-life of 48 h at 70°C, AmyB hasa half-life of only about 10 min at that temperature. However,in vivo chaperones, low-molecular-mass stabilizers, or othercytoplasmic compounds may have a stabilizing effect on AmyB.The precise physiological role of AmyB is not known, but theenzyme may be involved in the breakdown of maltooligosaccharidestransported into the cell or in the turnover of storage polysaccharides.

Many ${alpha}$ -amylases are known to be Ca²⁺ dependent. In the case ofAmyA, the addition of Ca²⁺ had a positive effect on activity.On the other hand, EDTA reduced the enzyme activity only undercertain conditions, namely, in Tris buffer. In HEPES and McIlvainebuffers, EDTA was unable to decrease the activity significantlyeven after incubation with the enzyme at elevated temperatures.The reason for the observed buffer-dependent effect of EDTAis unclear, but it may point to tightly bound Ca²⁺ that is releasedonly under certain circumstances.

Similarly, resistance to chelating agents was found for theA. gottschalkii type I pullulanase (2). While Ca²⁺ enhancesthe stability of the CGTase from A. gottschalkii, effects onactivity were not reported (23). The soda lake from which A.gottschalkii was originally isolated (Lake Bogoria, Kenya) isseverely depleted of Ca²⁺ (4), which makes a dependence of extracellularenzymes on loosely bound Ca²⁺ seem inappropriate. It has evenbeen reported for two Bacillus-related strains isolated fromsoda lakes in Ethiopia that amylase activity in the culturesupernatant was stimulated by EDTA and decreased by Ca²⁺ ions,possibly due to adaptation to the Ca²⁺-deficient environment(16).

Thermoalkaliphilic organisms are thus a promising source forchelating-reagent-resistant glycoside hydrolases, which areactive at alkaline pH values and tolerant of elevated temperatures.

ACKNOWLEDGMENTS

R. Sterner and R. Freudl are thanked for helpful discussions.We are grateful to H.-P. Klenk for his aid in sequence analysis.

Financial support from the Deutsche Bundesstiftung Umwelt (DBU)and the Deutsche Forschungsgemeinschaft (DFG; Li398/6-3) isgreatly appreciated.

FOOTNOTES

* Corresponding author. Mailing address: Institut für Mikrobiologie und Genetik, Georg-August-Universität Göttingen, Grisebachstr. 8, D-37077 Göttingen, Germany. Phone: 49-551-393795. Fax: 49-551-394897. E-mail: wliebl{at}gwdg.de.

Dedicated to H. G. Schlegel on the occasion of his 80th birthday.

REFERENCES

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