Branched alpha glucans
10626428 ยท 2020-04-21
Assignee
Inventors
- Joana Gangoiti Munecas (AG Groningen, NL)
- Sander Sebastiaan Van Leeuwen (AG Groningen, NL)
- Lubbert Dijkhuizen (AG Groningen, NL)
- Christina Vafeiadi (Lausanne, CH)
- Lisa Lamothe (Lausanne, CH)
Cpc classification
A23L29/225
HUMAN NECESSITIES
A61K31/715
HUMAN NECESSITIES
C12P19/18
CHEMISTRY; METALLURGY
A23L33/26
HUMAN NECESSITIES
A23V2002/00
HUMAN NECESSITIES
C12P19/04
CHEMISTRY; METALLURGY
A23L33/125
HUMAN NECESSITIES
C08B37/0009
CHEMISTRY; METALLURGY
A23L33/21
HUMAN NECESSITIES
A23L29/212
HUMAN NECESSITIES
International classification
C12P19/18
CHEMISTRY; METALLURGY
A23L33/21
HUMAN NECESSITIES
A23L33/125
HUMAN NECESSITIES
C12P19/04
CHEMISTRY; METALLURGY
C08B37/00
CHEMISTRY; METALLURGY
A61K31/715
HUMAN NECESSITIES
A23L29/212
HUMAN NECESSITIES
A23L29/225
HUMAN NECESSITIES
Abstract
The present invention relates to the field of poly- and oligosaccharides and their dietary effects. In particular it relates to a method of producing a branched -glucan. Further aspects of the invention are a branched -glucan comprising alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic linkages and having (1.fwdarw.4,6) branching points, a food composition, and the use of an -glucanotransferase enzyme for reducing the digestible carbohydrates of a starch containing food material.
Claims
1. A method of producing an -glucan with a ratio of branching of at least 8%, the method comprising; contacting an -glucanotransferase with a polysaccharide or oligosaccharide substrate having degree of polymerization (DP) of at least 3, wherein the polysaccharide or oligosaccharide comprises at least two (1.fwdarw.4) linked D-glucose residues at a non-reducing end and is selected from the group consisting of starch, starch derivatives, malto-oligosaccharides, amylose, amylopectin, maltodextrins, (1.fwdarw.4) glucans and combinations thereof, and wherein the -glucanotransferase comprises an amino acid sequence having at least 95% identity to SEQ ID NO:1.
2. The method according to claim 1, wherein the production of -glucan is stopped before the reaction between the polysaccharide or oligosaccharide substrate and the -glucanotransferase enzyme has reached completion.
3. The method according to claim 1, wherein the polysaccharide or oligosaccharide substrate is contacted with the -glucanotransferase enzyme at a temperature of between 30 C. and 75 C. and a pH of between 4.8 and 8.0.
4. The method according to claim 1, wherein the -glucan with a ratio of branching of at least 8% has less than 1.0% consecutive (1.fwdarw.6) glucosidic linkages.
5. The method according to claim 1, wherein the -glucan with a ratio of branching of at least 8% has less than 0.5% consecutive (1.fwdarw.6) glucosidic linkages.
6. The method according to claim 1, wherein the -glucan with a ratio of branching of at least 8% has no consecutive (1.fwdarw.6) glucosidic linkages.
7. The method according to claim 1, wherein the -glucanotransferase comprises an amino acid sequence having at least 96% identity to SEQ ID NO:1.
8. The method according to claim 1, wherein the -glucanotransferase comprises an amino acid sequence having at least 97% identity to SEQ ID NO:1.
9. The method according to claim 1, wherein the -glucanotransferase comprises an amino acid sequence having at least 98% identity to SEQ ID NO:1.
10. The method according to claim 1, wherein the -glucanotransferase comprises an amino acid sequence having at least 99% identity to SEQ ID NO:1.
11. The method according to claim 1, wherein the -glucanotransferase has an amino acid sequence of SEQ ID NO:1.
Description
DESCRIPTION OF THE DRAWINGS
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(4) The sequence identification numbers for the motifs I-IV of Azotobacter chroococcum NCIMB 8003 are SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, and SEQ ID NO:7 respectively. The sequence identification numbers for the motifs I-IV of Exiguobacterium sibiricum 255-15 are SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, and SEQ ID NO:11 respectively. The sequence identification numbers for the motifs I-IV of Exiguobacterium undae are SEQ ID NO:12, SEQ ID NO:13, SEQ ID NO:14, and SEQ ID NO:15 respectively. The sequence identification numbers for the motifs I-IV of Exiguobacterium antarcticum are SEQ ID NO:16, SEQ ID NO:17, SEQ ID NO:18, and SEQ ID NO:19 respectively. The sequence identification numbers for the motifs I-IV of Exiguobacterium acetylicum are SEQ ID NO:20, SEQ ID NO:21, SEQ ID NO:22, and SEQ ID NO:23 respectively. The sequence identification numbers for the motifs I-IV of Bacillus kribbensis are SEQ ID NO:24, SEQ ID NO:25, SEQ ID NO:26, and SEQ ID NO:27 respectively. The sequence identification numbers for the motifs I-IV of Bacillus coagulans DSM 1 are SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30, and SEQ ID NO:31 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus reuteri 121 (GtfB) are SEQ ID NO:32, SEQ ID NO:33, SEQ ID NO:34, and SEQ ID NO:35 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus reuteri ML1 (ML4) are SEQ ID NO:36, SEQ ID NO:37, SEQ ID NO:38, and SEQ ID NO:39 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus salivarius GJ-24 are SEQ ID NO:40, SEQ ID NO:41, SEQ ID NO:42, and SEQ ID NO:43 respectively. The sequence identification numbers for the motifs I-IV of Pediococcus pentosaceus are SEQ ID NO:44, SEQ ID NO:45, SEQ ID NO:46, and SEQ ID NO:47 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus plantarum are SEQ ID NO:48, SEQ ID NO:49, SEQ ID NO:50, and SEQ ID NO:51 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus reuteri DSM 20016 are SEQ ID NO:52, SEQ ID NO:53, SEQ ID NO:54, and SEQ ID NO:55 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus acidipiscis KCTC 13900 are SEQ ID NO:56, SEQ ID NO:57, SEQ ID NO:58, and SEQ ID NO:59 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus reuteri 180 are SEQ ID NO:60, SEQ ID NO:61, SEQ ID NO:62, and SEQ ID NO:63 respectively. The sequence identification numbers for the motifs I-IV of Lactobacillus reuteri 121 (GtfA) are SEQ ID NO:64, SEQ ID NO:65, SEQ ID NO:66, and SEQ ID NO:67 respectively. The sequence identification numbers for the motifs I-IV of Streptococcus mutants SI (GtfsI) are SEQ ID NO:68, SEQ ID NO:69, SEQ ID NO:70, and SEQ ID NO:71 respectively. The sequence identification numbers for the motifs I-IV of Leuconostoc mesenteroides are SEQ ID NO:72, SEQ ID NO:73, SEQ ID NO:74, and SEQ ID NO:75 respectively. The sequence identification numbers for the motifs I-IV of Bacillus sterothermophilus are SEQ ID NO:76, SEQ ID NO:77, SEQ ID NO:78, and SEQ ID NO:79 respectively. The sequence identification numbers for the motifs I-IV of Bacillus licheniformis are SEQ ID NO:80, SEQ ID NO:81, SEQ ID NO:82, and SEQ ID NO:83 respectively. The sequence identification numbers for the motifs I-IV of Bacillus sp. 707 are SEQ ID NO:84, SEQ ID NO:85, SEQ ID NO:86, and SEQ ID NO:87 respectively. The sequence identification numbers for the motifs I-IV of Halothermothrix orenii are SEQ ID NO:88, SEQ ID NO:89, SEQ ID NO:90, and SEQ ID NO:91 respectively.
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DETAILED DESCRIPTION OF THE INVENTION
(30) Consequently the present invention relates in part to a method of producing an -glucan with a ratio of branching of at least 8% (for example at least 12%) comprising contacting a polysaccharide or oligosaccharide substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units with an -glucanotransferase enzyme capable of cleaving (1.fwdarw.4) glucosidic linkages and making new alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic linkages with (1.fwdarw.4,6) branching points, wherein said -glucanotransferase is selected from the group consisting of GTFB, GTFC and GTFD types of enzyme (for example a GTFD type of enzyme), or a functional homolog thereof having the specified enzymatic activity. For example, the -glucanotransferase enzyme in the method of the invention may be capable of cleaving (1.fwdarw.4) glucosidic linkages and transferring malto-oligosaccharides up to DP5, resulting in the formation of single (1.fwdarw.6) linkages, in both alternating and branching patterns. Polysaccharides are polymeric carbohydrate molecules composed of long chains of monosaccharide units bound together by glycosidic linkages. Oligosaccharides are saccharide polymers containing a small number (typically three to nine) of monosaccharides. An example of a substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units is amylose.
(31) The method of the invention may comprise contacting a polysaccharide or oligosaccharide substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units with an -glucanotransferase enzyme capable of cleaving (1.fwdarw.4) glucosidic linkages and making new alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic linkages with (for example together with) (1.fwdarw.4,6) branching points without forming consecutive (1.fwdarw.6) glucosidic linkages, wherein said -glucanotransferase is selected from the group consisting of GTFB, GTFC and GTFD types of enzyme, or a functional homolog thereof having the specified enzymatic activity. In the present specification, the abbreviation GTF refers to glucanotransferase.
(32) The alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic linkages may be interspersed with some consecutive (1.fwdarw.4) glucosidic linkages, such a structure can also be described as chains of (1.fwdarw.4) linked D-glucose units interspersed with (1.fwdarw.6) glucosidic linkages. Single (1.fwdarw.6) glucosidic linkages between one or more (1.fwdarw.4) glucosidic linkages as may be formed in the method of the invention are sometimes referred to as bridging (1.fwdarw.6) linkages. The notation (1.fwdarw.4) may be used instead of (1.fwdarw.4) to refer to a 1.fwdarw.4 linkage, but these are equivalent, as are (1.fwdarw.6) and (1.fwdarw.6).
(33) The method of the invention may comprise contacting a polysaccharide or oligosaccharide substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units with an -glucanotransferase enzyme capable of cleaving (1.fwdarw.4) glucosidic linkages and making new (1.fwdarw.6) glucosidic linkages to form structures having chains of (1.fwdarw.4) linked D-glucose units interspersed with (1.fwdarw.6) glucosidic linkages and having (1.fwdarw.4,6) branching points, without forming consecutive (1.fwdarw.6) glucosidic linkages, wherein said -glucanotransferase is selected from the group consisting of GTFB, GTFC and GTFD types of enzyme, or a functional homolog thereof having the specified enzymatic activity.
(34) In the context of the present invention, the ratio of branching is defined as the total number of branching anhydroglucose units (AGU), i.e. AGU being bound to three other units, with respect to the total number of AGU of a molecule. The ratio of branching can be determined by methods known in the art, such as methylation with gas chromatography. The -glucan produced by the method of the invention may have a ratio of branching of at least 8%, for example at least 10%, for example at least 15%.
(35) The -glucan produced by the method of the invention may comprise at least one (1.fwdarw.4) glucosidic linkage adjacent to an (1.fwdarw.6) glucosidic linkage and at least one (1.fwdarw.4,6) branching point. The -glucan produced by the method of the invention may comprise alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic linkages and have (1.fwdarw.4,6) branching points, for example the -glucan produced by the method of the invention may comprise between 40 and 50 percent consecutive (1.fwdarw.4) glucosidic linkages, between 12 and 21 percent single (1.fwdarw.6) glucosidic linkages in alternating pattern and between 8 and 25 percent (1.fwdarw.4,6) branching points, for example between 12 and 21 percent (1.fwdarw.4,6) branching points, for example between 15 and 20 percent (1.fwdarw.4,6) branching points. The -glucan produced by the method of the invention may have less than 1% consecutive (1.fwdarw.6) glucosidic linkages, for example it may have less than 0.5% consecutive (1.fwdarw.6) glucosidic linkages, for further example it may have no consecutive (1.fwdarw.6) glucosidic linkages.
(36) The -glucanotransferase in the method of the invention may comprise an amino acid sequence having at least 80% identity to SEQ ID NO:1 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:1). The -glucanotransferase in the method of the invention may consist of an amino acid sequence having at least 80% identity to SEQ ID NO:1 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:1).
(37) TABLE-US-00001 (SEQIDNO:1) mraspsqffaisllsiaisgllsgaavaapaptaleqvpd gkggvkwqevthdasaeeeqkgqdpkkflgiqaittepdg svkvemgkpevrqpasgdvfvsnekldehvifqafalyqp ndnatykaltenapqlaqwgitdvwspppyraasdskyge gyaiadrydlgaydkgptkygtadelkaaigalhnndiri qvdvvpnqiiglnerhvlpvtgvdmygkpmnpfldhylys tyskgsapgqaehgvikewdyfhfhgtttqyqglfrvlsd anstlyrylgpnhpenylpaflaesdaakygkintidgyl ladtwfavenaesenavyaplflyyeeprngvveqtfmdf arengytgsdediratmlaelrmtpnpigplmdeylaaqp gyskkseddakvtalrydgpendashigtnvldfeflvgn dldtiredvqqeqlnwqkylldfgfdgfridaashintdm lrdevtqrlnhfagedvnehlsyiesyvtqqvdflqsnny gqmamdagpfsglmfsfgrdwaplryafeaslidrvnggp alpnwsfvnnhdqehnilvtvplteeeaggyepnsqpyel rqlekydadrnsvekqwaphnvpamyaillttkdtvptvf ygdmfvsskpymstptpyrddivnilklrkqfakgeqvir yensntgsngedlvsnirlgndrktgvavvagnnpaldtt itvdmgaqhrnqwfvdamgyqperlktdkdgrltvqvkgt qnvdvkgylaawvpdlqaqe
(38) The -glucanotransferase in the method of the invention may be an Azotobacter chroococccum GTFD enzyme for example the -glucanotransferase in the method of the invention may be an Azotobacter chroococccum NCIMB 8003 GTFD enzyme. The method of the invention for producing an -glucan with a ratio of branching of at least 8% may comprise contacting a polysaccharide or oligosaccharide substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units with an Azotobacter chroococccum GTFD enzyme.
(39) A further aspect of the invention provides a method for producing an -glucan with a ratio of branching of at least 8%, the method comprising contacting a polysaccharide or oligosaccharide substrate, comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units, with an -glucanotransferase enzyme comprising (for example consisting of) an amino acid sequence having at least 80% identity to SEQ ID NO:92 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:92). SEQ ID NO:92 is the sequence of Paenibacillus beijingensis DSM 24997 GFTD enzyme, Gen bank accession WP_052702730.1.
(40) The -glucanotransferase in the method of the invention may comprise an amino acid sequence having at least 80% identity to SEQ ID NO:92 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:92). The -glucanotransferase in the method of the invention may consist of an amino acid sequence having at least 80% identity to SEQ ID NO:92 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:92).
(41) The -glucanotransferase in the method of the invention may be a Paenibacillus beijingensis GTFD enzyme for example the -glucanotransferase in the method of the invention may be a Paenibacillus beijingensis DSM 24997 GFTD enzyme. Paenibacillus beijingensis DSM 24997 is the type strain of P. beijingensis, also known as ACCC 03082, and may be obtained from Leibniz-Institut DSMZDeutsche Sammlung von Mikroorganismen and Zellkulturen GmbH. The method of the invention for producing an -glucan with a ratio of branching of at least 8% may comprise contacting a polysaccharide or oligosaccharide substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units with a Paenibacillus beijingensis GTFD enzyme.
(42) An aspect of the invention provides a method for producing an -glucan with a ratio of branching of at least 8%, the method comprising contacting a polysaccharide or oligosaccharide substrate, comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units, with -glucanotransferase comprising an amino acid sequence having at least 80% identity to SEQ ID NO:92.
(43) The substrate in the method of the invention may have a degree of polymerization of at least three, for example it may comprise at least three D-glucose units. The degree of polymerization is the number of monomeric units in a polymer or oligomer molecule. For example, the substrate in the method of the invention may have a degree of polymerization of at least four, for example it may comprise at least four D-glucose units. The substrate in the method of the invention may be selected from the group consisting of starch (for example waxy starch or high amylose starch), starch derivatives, malto-oligosaccharides, amylose, amylopectin, maltodextrins, (1.fwdarw.4) glucans and combinations thereof. Starch derivatives are prepared by physically, enzymatically, or chemically treating native starch to change its properties.
(44) The substrate in the method of the invention may be comprised within another material, for example the substrate may be starch provided in the form of flour. It is advantageous to be able to convert polysaccharides or oligosaccharides comprised within food ingredients into -glucans with lower digestibility, for example branched -glucans. Such a conversion may increase the fibre content of the ingredients and/or may aid in reducing the calorie content of the ingredients. The method of the invention may be performed as part of a food processing operation, for example the -glucanotransferase enzyme may be applied to food ingredients during a process to produce a food product. The substrate may be comprised within a material which already has a positive nutritional profile, for example the substrate may be comprised within whole grain flour.
(45) The extent to which the polysaccharide or oligosaccharide substrate may be converted by the -glucanotransferase enzyme in the method of the invention can be adjusted by limiting the time of reaction. Partially converted substrates will provide different physical properties. The production of -glucan in the method of the invention may be stopped before the reaction between the substrate and the -glucanotransferase enzyme has reached completion, for example it may be stopped by denaturing (e.g. by heat) or removing the enzyme.
(46) The -glucanotransferase enzyme in the method of the invention may be immobilized, for example immobilized before contacting the polysaccharide or oligosaccharide substrate. Such immobilization techniques are well known in the art. Removal of the enzyme (discussed above) may be facilitated by immobilization of the enzyme. Immobilization techniques may be selected from the group consisting of covalent binding, entrapment, physical adsorption, cross-linking and combinations of these. In immobilization by covalent binding, enzymes are covalently linked to a support through the functional groups in the enzymes that are not essential for the catalytic activity. Oxides materials such as alumina, silica, and silicated alumina can be used for covalent binding of the enzyme. In immobilization by entrapment the enzyme is localized within the lattice of a polymer matrix or membrane. Entrapment methods are classified into five major types: lattice, microcapsule, liposome, membrane, and reverse micelle. The enzyme is entrapped in the matrix of various synthetic or natural polymers. Alginate, a naturally occurring polysaccharide that forms gels by ionotropic gelation is one such immobilization matrix. Immobilization by physical adsorption is the simplest and the oldest method of immobilizing enzymes onto carriers. Immobilization by adsorption is based on the physical interactions between the enzymes and the carrier, such as hydrogen bonding, hydrophobic interactions, van der Waals force, and their combinations. Adsorption is generally less disruptive to the enzymes than chemical means of attachment. Immobilization by cross-linking utilizes bi- or multifunctional compounds, which serve as the reagent for intermolecular cross-linking of the enzymes. Cross-linking may be used in combination with other immobilization methods such as adsorption or entrapment.
(47) The polysaccharide or oligosaccharide substrate may be contacted with an -glucanotransferase enzyme in the method of the invention at a temperature of between 30 C. and 75 C. (for example between 40 C. and 75 C., for example between 50 C. and 70 C., for example between 35 C. and 45 C.) and a pH of between 4.8 and 8.0 (for example between 5.5 and 7.5, for example between 6.0 and 7.0).
(48) In a further embodiment the present invention pertains to an -glucan comprising alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic linkages and having (1.fwdarw.4,6) branching points wherein the -glucan has a ratio of branching of at least 12% (for example at least 15%), has more than 1 wt. % maltopentose units and has an average molecular mass between 110.sup.6 Da and 4010.sup.6 Da, for example, an average molecular mass between 510.sup.6 Da and 3010.sup.6 Da, for example, an average molecular mass between 1010.sup.6 Da and 2010.sup.6 Da. The -glucan according to the invention may comprise between 40 and 50 percent consecutive (1.fwdarw.4) glucosidic linkages, between 12 and 21 percent single (1.fwdarw.6) glucosidic linkages in alternating pattern and between 12 and 25 percent (1.fwdarw.4,6) branching points, for example between 12 and 21 percent (1.fwdarw.4,6) branching points, for example between 15 and 20 percent (1.fwdarw.4,6) branching points. The -glucan according to the invention may have less than 1% consecutive (1.fwdarw.6) glucosidic linkages, for example it may have less than 0.5% consecutive (1.fwdarw.6) glucosidic linkages, for further example it may have no consecutive (1.fwdarw.6) glucosidic linkages. The -glucan of the invention is similar to the reuteran synthesized by the L. reuteri 121 GTFA glucansucrase from sucrose, regarded as a health promoting food ingredient, but has some important differences. The ratio of branching is higher, for example in the samples analysed in table 3 it can be seen that Azotobacter chroococcum NCIMB 8003 GTFD enzyme produces 18% branching compared to 11% for L. reuteri 121 GTFA enzyme. The more branching is present in an -glucan, the less access is provided to digestive enzymes and so the -glucan could present a lower digestibility. The -glucan of the invention also comprises maltopentose units in its structure (see
(49) The -glucan of the invention may have (1.fwdarw.4,6) branching points, a ratio of branching of at least 12%, more than 1 wt. % maltopentose units, less than 1% consecutive (1.fwdarw.6) glucosidic linkages (for example less than 0.5% consecutive (1.fwdarw.6) glucosidic linkages, for further example no consecutive (1.fwdarw.6) glucosidic linkages), an average molecular mass between 110.sup.6 Da and 4010.sup.6 Da and may comprise structures (for example linear structures) having chains of (1.fwdarw.4) linked D-glucose units interspersed with (1.fwdarw.6) glucosidic linkages. The -glucan of the invention may comprise at least 1% of structures having chains of (1.fwdarw.4) linked D-glucose units interspersed with (1.fwdarw.6) glucosidic linkages, for example at least 10% structures having chains of (1.fwdarw.4) linked D-glucose units interspersed with (1.fwdarw.6) glucosidic linkages, for further example at least 20% structures having chains of (1.fwdarw.4) linked D-glucose units interspersed with (1.fwdarw.6) glucosidic linkages. The -glucan of the invention may have at least 5% (1.fwdarw.6) glucosidic linkages. The Paenibacillus beijingensi GTFD enzyme synthesizes a high and a low molecular mass polymer from amylose V (see
(50) In a further aspect, the invention provides an -glucan obtainable (for example obtained) by contacting a polysaccharide or oligosaccharide substrate comprising at its non-reducing end at least two (1.fwdarw.4) linked D-glucose units with an -glucanotransferase enzyme comprising an amino acid sequence having at least 80% identity to SEQ ID NO:1, or at least 80% identity to SEQ ID NO:92.
(51) The -glucan of the invention can be regarded as a dietary fiber. Due to its highly branched structure, the -glucan will resist enzymatic degradation in the upper gastrointestinal tract and end up in the large intestine where it can be fully fermented by the colonic microflora. In addition, such dietary fibres enhance satiety in humans or animals. Blood sugar levels rise after a meal. As the -glucans of the invention display reduced digestibility compared to materials such as starch, meals prepared containing them will cause a reduced blood glucose response compared to the equivalent meal with starch, and will provoke a lower insulin response. A composition comprising the -glucan of the invention may be for use in the control of postprandial blood glucose and insulin levels in a subject. The subject may be a human or a pet. A composition comprising the -glucan of the invention may be for use in the treatment or prevention of a disorder linked to an increase in postprandial blood glucose and insulin levels in a subject. The disorder may be selected from the group consisting of diabetes, for example gestational diabetes; impairment of glucose metabolism; hyperinsulinemia or insulin resistance. The subject may be a diabetic or pre-diabetic human or pet.
(52) Typically, postprandial hyper-insulinemia may promote the development of insulin resistance, metabolic syndrome, glucose intolerance and type-2 diabetes [Kopp W., Metabolism. 2003, July; 52(7):840-844]. Lowering the insulin demand after a meal however, can reduce on one hand the deterioration of the glycemic control in type-2 diabetes and on the other hand reduce the risk of developing type-2 diabetes in predisposed subjects.
(53) A pre-diabetic patient is a subject showing insulin resistance or impaired glucose metabolism and is predisposed, for example by family history, lifestyle or genetics, for developing diabetes later in life. Reducing insulin secretion reduces the risk of the pancreas becoming exhausted in the long term, and so is beneficial for management of the pancreas in pre-diabetes or patients with metabolic disorders. The use of a composition comprising the -glucan of the invention would consequently reduce the risk and/or the development of diabetes, impaired glucose metabolism, hyperinsulinemia or insulin resistance in those subjects.
(54) Prevalence of diabetes, insulin resistance or glucose intolerance is mostly observed in adult humans. However, more and more children are affected, or predisposed or at risk of developing such a disorder later in life. Hence, advantageously, prevention and/or treatment of those disorders is started already in young age. Alternatively, and similarly as observed with humans; diabetes, hyperinsulinemia or insulin resistance are more and more widespread among animals, particularly with animals kept as pet animals. Hence, the invention also pertains to cats and dogs.
(55) A composition comprising the -glucan of the invention may be for non-therapeutic use to decrease plasma postprandial glucose and insulin levels. It is advantageous that a composition comprising the -glucan of the invention can also be administered to subjects, for example healthy subjects, which may be at risk of developing diabetes type-2, insulin resistance or glucose intolerance at some later time. A composition comprising the -glucan of the invention, as disclosed herein, provides a reduced insulin level after consumption. Many healthy people desire to lose weight. Consuming meals which contain dietary fibre can increase satiety and therefore help people consume fewer digestible calories. A composition comprising the -glucan of the invention may be for non-therapeutic use to lose weight.
(56) Another aspect of the invention relates to a food composition comprising the -glucan of the invention. The food composition may for example comprise between 1 and 20 wt. % of the -glucan of the invention. The food composition may be a beverage, for example a powdered beverage mix or a beverage creamer; a breakfast cereal; a pet food product; a baked dough product, for example a bread, a pizza or a filled savoury turnover; or a confectionery product. The confectionery product may be a frozen confectionery product such as an ice-cream; a baked confectionery product such as a biscuit, for example a filled biscuit or wafer; a chocolate confectionery product; or a sugar-style confectionery product such as a gum, a jelly, a hard-boiled sweet or a chewy sweet. The term sugar-style confectionery product or sugar-style candy refers to confectionery products which would traditionally have been based on sugar, but may be manufactured with alternative sweeteners and/or sugar substitutes.
(57) In a further embodiment, the invention provides for the use of a GTFD -glucanotransferase enzyme for reducing the digestible carbohydrates of a food material. The invention provides for the use of an -glucanotransferase enzyme that comprises an amino acid sequence having at least 80% identity to SEQ ID NO:1 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:1), or has an amino acid sequence of SEQ ID NO:1, for reducing the digestible carbohydrates of a food material, for example a starch-containing food material. In the scope of the current invention, digestible carbohydrates correspond to the fraction of the total carbohydrates that is digestible and available to provide energy to body cells.
(58) The invention further provides for the use of a GTFD -glucanotransferase enzyme that comprises an amino acid sequence having at least 80% identity to SEQ ID NO:92 (for example at least 90, 95, 96, 97, 98, or 99% identity to SEQ ID NO:92), or has an amino acid sequence of SEQ ID NO:92, for reducing the digestible carbohydrates of a food material, for example a starch-containing food material.
(59) The invention provides for the use of a GTFD -glucanotransferase enzyme for reducing the glycemic index of a food material, for example -glucanotransferase enzyme that comprises an amino acid sequence having at least 80% identity (for example at least 90, 95, 96, 97, 98, or 99% identity) to SEQ ID NO:1 or SEQ ID NO:92. The glycemic index is a number associated with a particular type of food that indicates the food's effect on a person's blood glucose (also called blood sugar) level. A value of 100 represents the standard, an equivalent amount of pure glucose.
(60) Those skilled in the art will understand that they can freely combine all features of the present invention disclosed herein. In particular, features described for the method of the present invention may be combined with the product of the present invention and vice versa. Further, features described for different embodiments of the present invention may be combined. Where known equivalents exist to specific features, such equivalents are incorporated as if specifically referred to in this specification. Further advantages and features of the present invention are apparent from the figures and experimental section.
EXPERIMENTAL SECTION
Introduction
(61) Glycoside Hydrolase (GH) family 70 originally was established for glucansucrase (GSs) enzymes (http://www.cazy.org/), which solely are found in lactic acid bacteria (Lombard et al., 2014). GSs use sucrose to synthesize a diversity of linear and branched -glucans, differing in the type of glycosidic linkages, the degree and type of branching, the length of the glucan chains, molecular mass, and the conformation of the polymers. Depending on the main glucosidic linkage present in their glucans products, they can be divided into dextran [(1.fwdarw.6) linkages], mutan [(1.fwdarw.3) linkages], reuteran [(1.fwdarw.4) and (1.fwdarw.6) linkages], and alternan [alternating (1.fwdarw.3) and (1.fwdarw.6) linkages]. Enzymes from GH70 belong to clan GH-H (also known as -amylase superfamily), together with enzymes from families GH13 (mainly starch modifying enzymes) and GH77 (e.g. 4--glucanotransferases) (Stam et al., 2006). All GH-H members employ a similar catalytic mechanism, involving a covalent glucosyl intermediate and retention of the -configuration in their products, but they vary widely in their product and reaction specificity.
(62) To date, 60 GS enzymes have been biochemically characterized and three-dimensional structures are available for four proteins with different product specificity (Vujicic-Zagar et al., 2010; Ito et al., 2011; Brison et al., 2012; Pijning et al., 2012). These crystal structures showed that GSs are structurally similar to the closely related GH13 and GH77 starch modifying enzymes, confirming earlier secondary-structure predictions (MacGregor et al., 1996; 2001). However, GSs also possess unique structural features. Firstly, compared to GH13 and GH77 enzymes, their catalytic (/).sub.8-barrel domain is circularly permuted. As a consequence, in GSs the order of the four signature sequence motifs I-IV of clan GH-H is II-III-IV-I (
(63) Recently, a GH70 subfamily of enzymes inactive on sucrose, but displaying clear hydrolase/transglycosylase activity on malto-oligosaccharides (MOS) and starch has been identified, which also reflects the evolutionary relationships between families GH70 and GH13 (Kralj et al., 2011). Members of this subfamily have clear sequence similarity with GS enzymes, and are only found in lactic acid bacteria. The Lactobacillus reuteri 121 GTFB enzyme is the first characterized member of this subfamily cleaving (1.fwdarw.4) linkages and synthesizing (1.fwdarw.6) linkages, designated as a 4,6--glucanotransferase (4,6--GT) enzyme. As a result of GTFB enzyme activity, linear isomalto-/malto-polysaccharides (IMMPs) are produced which consist of linear (1.fwdarw.6)-glucan chains attached to the non-reducing ends of MOS or starch fragments. IMMPs represent a new type of starch derived soluble dietary fiber according to in vitro studies, and as such they are potentially valuable food ingredients (Bai et al., 2015a; Dobruchowska et al., 2012; Dijkhuizen et al., 2010; Leemhuis et al., 2014). The exact in vivo role of GTFB-like enzymes remains unknown. It should be noted that the gtfB gene was identified upstream of the gtfA gene from L. reuteri 121 encoding a regular GH70 glucansucrase that converts sucrose into reuteran, a branched glucan with alternating (1.fwdarw.4) and (1.fwdarw.6) linkages) (Kralj et al., 2002; van Leeuwen et al., 2008a, Dobruchowska et al., 2013).
(64) More recently a second GH70 subfamily with 4,6--glucanotransferase activity in non-lactic acid bacteria has been identified and the Exiguobacterium sibiricum 255-15 GTFC enzyme (Gangoiti et al., 2015) characterized. Exiguobacterium is a genus of bacilli and the data shows that biochemically this GTFC enzyme is rather similar to the L. reuteri GTFB enzymes. A main difference observed is that this GTFC enzyme synthesizes IsoMalto-/Malto-Oligosaccharides (IMMOs), instead of a (modified) polymer (IMMP) from malto-oligosaccharides and amylose V. Regarding their amino acid sequences, the L. reuteri 121 GTFB and the E. sibiricum GTFC share only 30% identity, but they display high conservation in their signature motifs I-IV. However, the order of these conserved motifs in GTFC enzymes is I-II-III-IV reflecting their non-permuted domain organization, similar to GH13 proteins but differing from the permuted order II-III-IV-I characteristic for glucansucrases and GTFB-like 4,6--glucanotransferases (
(65) This experimental section reports the biochemical characterization of a novel GH70 enzyme with unique product specificity and a different microbial origin, Azotobacter chroococcum NCIMB 8003. This protein was designated GTFD and resembles 4,6--glucanotransferases in using maltodextrins and starch as substrates. However, the A. chroococcum GTFD enzyme catalyzes the synthesis of a high molecular mass and relatively highly branched -glucan with alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic bonds from amylose. This product does not contain consecutive (1.fwdarw.6) linkages, clearly differing from the IMMPs and IMMOs synthesized by the L. reuteri 121 GTFB and E. sibiricum GTFC, respectively. The structure of the polymer formed by the A. chroococcum GTFD enzyme is more similar to that of the reuteran synthesized by the L. reuteri 121 GTFA glucansucrase from sucrose (Kraj et al., 2004; van Leeuwen et al., 2008a; Dobruchowska et al., 2013). With the discovery of this novel Azotobacter GTFD 4,6--glucanotransferase it appears that the distribution of GH70 enzymes is not limited to Gram-positive bacteria. A. chroococcum NCIMB 8003 is a soil-dwelling, N.sub.2 fixing Gram-negative bacterium that forms thick-walled cysts. Based on the analysis of its recently elucidated genome, this bacterium was predicted to produce extracellular polysaccharides such as alginate, levan and cellulose (Robson et al., 2015). Our work suggests that A. chroococcum also is able to synthesize a reuteran-like -glucan from starch/maltodextrins. The in vivo role of the polymer produced by the A. chroococcum GTFD 4,6--glucanotransferase enzyme remains to be investigated.
(66) A. chroococcum GTFD showed 48% identity in amino acid sequence to a hypothetical GH70 enzyme encoded by Paenibacillus beijingensis DSM 24997 (Genbank accession WP_052702730.1). With the aim of further expanding the repertoire of starch-converting GH70 family enzymes, the GTFD enzyme of the plant-growth promoting rhizobacterium Paenibacillus beijingensis DSM 24997 was characterized. Our data shows that the P. beijingensis GTFD is also a reuteran-like polymer-forming 4,6--GTase, providing the first example of this novel reaction and product specificity in a Gram-positive bacterium. Besides, differences between the products synthesized by the action of the A. chroococcum GTFD and P. beijingensis GTFD were found, enlarging the range of reuteran-like polymers that can be synthesized from amylose. Finally, A. chroococcum GTFD and P. beijingensis GTFD isolated reuteran-like polymers, and the reaction mixtures obtained from starch incubations were subjected to in vitro digestibility studies with digestive enzymes (porcine pancreatin and rat intestinal powder extracts) in other to evaluate the potential use of these enzymes for the production of less easily digestible starchy food.
(67) Materials and Methods
(68) Phylogenetic Analysis
(69) The E. sibiricum 255-15 sequence was retrieved from the GH70 database (http://www.cazy.org) and used as query in BLASTp searches (http://www.ncbi.nlm.nih.gov/BLAST/). Phylogenetic analysis was performed using MEGA, version 6 (Tamura et al., 2013) with a total of 71 amino acid sequences corresponding to representative GH70 and GH13 sequences identified via BLASTp. The GenBank accession numbers of the sequences used in this section are listed in Table 1. Sequences were aligned by MUSCLE, using default parameters. A phylogenetic tree was constructed by the Maximum Likelihood method based on the JTT matrix based model using in MEGA6. Partial deletion of the positions containing alignment gaps and missing data was conducted. Statistical confidence of the inferred phylogenetic relationships was assessed by performing 1,000 bootstrap replicates.
(70) TABLE-US-00002 TABLE 1 GenBank accession numbers of the family GH70 and GH13 protein sequences used in the phylogenetic tree of FIG. 2. GTFC-like proteins gi|501339877|dextransucrase Exiguobacterium sibiricum 255-15 gi|654644457|dextransucrase Exiguobacterium undae gi|504784268|dextransucrase Exiguobacterium antarcticum B7 gi|657229007|dextransucrase Exiguobacterium acetylicum gi|737429885|dextransucrase Exiguobacterium sp. RIT341 gi|737339900|dextransucrase Bacillus kribbensis gi|737335335|dextransucrase partial Bacillus coagulans gi|757632476|dextransucrase partial Bacillus coagulans gi|335366490|dextransucrase Bacillus coagulans 2-6 gi|753712235|alpha amylase catalytic domain protein Bacillus coagulans DSM 1 ATCC 7050 GTFD proteins .fwdarw. gi|747128849|dextransucrase Azotobacter chroococcum NCIMB 8003 GFTB- gi|489780009|dextransucrase partial Lactobacillus fermentum ATCC 14931 like gi|490699763|dextransucrase partial Lactobacillus fermentum 28-3-CHN protei gi|738781828|glycosyl hydrolase family 70 partial Pediococcus pentosaceus gi|767167586|glycosyl hydrolase family 70 Lactobacillus delbrueckii gi|312280789|dextransucrase Lactobacillus delbrueckii subsp. bulgaricus ND02 gi|357208772|putative glucansucrase Lactobacillus reuteri gi|737661728|hypothetical protein partial Lactobacillus acidipiscis gi|754206103|dextransucrase partial Lactobacillus sanfranciscensis gi|189485784|inactive glucansucrase Lactobacillus reuteri gi|752446660|hypothetical protein partial Lactobacillus plantarum gi|335350722|inactive glucansucrase Lactobacillus salivarius GJ-24 gi|148531598|dextransucrase Lactobacillus reuteri DSM 20016 Glucansucrases gi|51574161|glucansucrase Lactobacillus parabuchneri gi|118432573|dextransucrase Oenococcus oeni ATCC BAA-1163 gi|599001939|glucosyltransferase GTFG Lactobacillus sucicola DSM 21376 JCM 15457 gi|68160983|Ir1943 Lactobacillus reuteri gi|7684297|glucosyltransferase Streptococcus oralis gi|146741366|glucosyltransferase Streptococcus criceti gi|390484468|glucansucrase Weissella confusa LBAE C39-2 gi|3130095|glucosyltransferase-SI Streptococcus mutans gi|251825496|glucansucrase Leuconostoc lactis gi|217330914|glucansucrase Weissella cibaria gi|444737522|dextransucrase Lactobacillus curvatus gi|145666440|dextransucrase Lactobacillus reuteri gi|632814081|glucosyltransferase-I Lactobacillus kunkeei EFB6 gi|599000389|glucosyltransferase GTFG Lactobacillus sucicola DSM 21376 JCM 15457 gi|51574173|glucansucrase Lactobacillus reuteri gi|296470401|dextransucrase Leuconostoc citreum gi|22138845|glucosyltransferase Streptococcus sobrinus gi|679092076|alternansucrase Leuconostoc citreum gi|51574154|glucansucrase Lactobacillus reuteri gi|374074331|chain A Crystal Structure Of Leuconostoc Mesenteroides Nrrl B-1299 N GH13 proteins gi|755167313|alpha-amylase Streptococcus pneumoniae gi|565861005|alpha-amylase Streptococcus mitis gi|494939858|alpha-amylase Bacteroides intestinalis DSM gi|492283664|alpha-amylase Bacteroides fragilis gi|806522612|alpha-amylase Parabacteroides goldsteinii DSM 19448 WAL 12034 gi|446718150|alpha-amylase Escherichia fergusonii gi|737197682|alpha-amylase Bacillus coagulans gi|499280363|alpha-amylase Agrobacterium tumefaciens gi|753800608|alpha-amylase Odoribacter splanchnicus gi|657310130|cytoplasmic alpha-amylase Escherichia coli gi|8250115|maltohexaose-forming alpha-amylase Geobacillus stearothermophilus gi|228609270|glucan 14-alpha-maltohexaosidase Bacillus cereus MM3 gi|228615225|glucan 14-alpha-maltohexaosidase Bacillus cereus AH621 gi|2642326|alpha amylase Geobacillus stearothermophilus gi|507056452|alpha-amylase Bacillus cereus gi|511013757|alpha-amylase Bacteroides thetaiotaomicron gi|1351934|alpha-amylase Geobacillus stearothermophilus gi|504109272|alpha-amylase Klebsiella pneumoniae gi|652433783|alpha-amylase Exiguobacterium sibiricum gi|228773147|glucan 14-alpha-maltohexaosidase Bacillus thuringiensis serovar tochigiensis BGSC 4Y1 gi|652438445|alpha-amylase Exiguobacterium undae gi|506403824|alpha-amylase B Halothermothrix orenii H 18 gi|782762336|cytoplasmic alpha-amylase Klebsiella pneumoniae gi|518247975|hypothetical protein Anoxybacillus kamchatkensis gi|763044452|alpha-amylase Bacillus licheniformis S 16 gi|647494625|alpha-amylase Bacillus licheniformis gi|304346690|glucan 14-alpha-maltohexaosidase Paenibacillus curdlanolyticus YK9 gi|113762|Maltohexaose-producing amylase Bacillus sp. 707
(71) Protein Sequence Analysis
(72) Signal peptide cleavage site was predicted using the Signal P4.1 server (http:/www.cbs.dtu.dk/services/SignalP/). Conserved domain searches were performed using the Pfam server (http://pfam.sanger.ac.uk/). Pairwise sequence comparison between the functional regions identified by the Pfam server and the Lactobacillus reuteri 121 GTFB and Exiguobacterium sibiricum 255-15 GTFC sequences were performed using Jalview (Waterhouse et al., 2009). Alternatively, multiple amino acid sequence alignments were generated with the ClustalW2 program (http://www.ebi.ac.uk/Tools/msa/clustalw2) and visualized by using Jalview (Waterhouse et al., 2009).
(73) Cloning of the gtfD Gene from A. chroococcum
(74) The DNA fragment coding for the full length GTFD protein (GenBank entry AJE22990.1, amino acids 29-780) was amplified from A. chroococcum NCIMB 8003 chromosomal DNA with Phusion DNA polymerase (Finnzyme) and cloned into a modified pET15b vector using ligation-independent cloning (LIC). For LIC cloning the following primer pairs with 5 extensions (in bold) were used for PCR amplification: Forward CAGGGACCCGGTGCACCGGCCCCCACGGCGCTCG (SEQ ID NO: 2) and Reverse CGAGGAGAAGCCCGGTTACTCCTGGGCCTGGAGGTCCGGAACCC (SEQ ID NO: 3). Basically, the Kpnl-digested vector and gtfD PCR product were isolated from gel and then treated with T4 DNA polymerase (New England Biolabs) in the presence of dTTP and dATP, respectively. The two reaction products were mixed together in a 1:4 molar ratio, and the mixture was used to transform Escherichia coli DH5a cells (Phabagen). This resulted in a gtfD construct containing an N-terminal His6-tag cleavable by a 3C protease. The constructed expression vector pET15b/gtfD was transformed into host E. coli BL21 Star (DE3). The gene sequence was verified by nucleotide sequencing (LGC genomics, Berlin, Germany).
(75) Protein Expression and PurificationA. chroococcum
(76) E. coli BL21 Star (DE3) harboring the gtfD gene of A. chroococcum NCIMB 8003 was cultured in Luria Broth medium supplemented with ampicillin (100 g ml.sup.1) at 37 C. and 230 rpm. When the cultures reached OD6000.6, the inducer isopropyl--D-1-thiogalactopyranoside (IPTG) was added to a final concentration of 0.1 mM, and cultivation was continued for 24 h at 16 C. The cells were harvested by centrifugation (10,000 g, 20 min) and subsequently lysed with B-PER protein extraction reagent (Thermo Scientific, Pierce). After centrifugation (15,000 g, 20 min) the cell-free extracts with soluble GTFD protein were subjected to Ni-IMAC chromatography. Following washing with 20 mM Tris-HCl (pH 8.0) and 1 mM CaCl.sub.2 the proteins were eluted with 200 mM imidazole in the same buffer. The GTFD containing fractions were concentrated and exchanged into 20 mM Tris-HCl buffer 1 mM CaCl.sub.2 (pH 8.0) in a stirred ultrafiltration unit (Amicon, Beverly, Mass.) on a 30,000 molecular mass cut-off membrane. Purity was checked by SDS-PAGE, and protein concentrations were determined using a Nanodrop 2000 spectrophotometer (Isogen Life Science, De Meern, The Netherlands).
(77) Cloning of the P. beijingensis GTFD Gene
(78) The 2241-bp DNA fragment coding for the full-length GTFD enzyme without its putative signal peptide-encoding sequence (amino acids 31 to 776) was amplified by PCR using Phusion DNA polymerase (Finnzyme, Helsinki, Finland) and the P. beijingensis chromosomal DNA (DSM 24997) as the template. The PCR primers used for amplifying the GTFD gene incorporated 5 extensions (in bold) to facilitate the ligation-independent (LIC) cloning and were: PbF (5 CAGGGACCCGGTGCGGAAAGCAATGCGAAAGG 3) (SEQ ID NO: 93) and PbR (5 CGAGGAGAAGCCCGGTTAATTGCTAAACCGTCTTAATGCTTTATTC 3) (SEQ ID NO: 94). The GTFD PCR product was cloned into a modified pET15b vector by ligation-independent cloning (LIC), resulting in a GTFD construct containing an N-terminal His6-tag cleavable by a 3C protease. The constructed expression vector pET15/PbGTFD was transformed into host E. coli BL21 Star (DE3). The construct was confirmed by sequencing (GATC, Cologne, Germany).
(79) Recombinant P. beijingensis GTFD Protein Production in E. coli and Purification
(80) Escherichia coli BL21 Star (DE3) carrying pET15/PbGTFD was grown in 500-ml LB medium containing 100 g ml.sup.1 ampicillin in a rotary shaker (37 C., 220 rev min.sup.1) to an optical density at 600 nm of 0.4-0.6. Expression of recombinant GTFD was induced by adding isopropyl--d-thiogalactopyranoside (IPTG) at a final concentration of 0.1 mM, and cultivation was continued at 16 C. for 20 h. Cells were harvested by centrifugation (10,000 g20 min) and then disrupted with B-PER lysis reagent (Thermo Scientific, Pierce). After centrifugation (15,000 g20 min), the soluble GTFD protein was purified from the cell-free extract by His-tag affinity chromatography using Ni.sup.2+nitrilotriacetate (Ni-NTA) as column material (Sigma-Aldrich). After washing the column with 25 mM Tris-HCl (pH 8.0), 1 mM CaCl.sub.2, bound proteins were eluted with 200 mM imidazole in the same buffer and the imidazole was removed by use of a stirred ultrafiltration unit (Amicon, Beverly, Mass.) with a 30,000 molecular weight cut off. Purity and homogeneity of the purified protein was analyzed by SDS-PAGE and the amount of protein in the enzyme solutions was routinely determined with a (Nanodrop 2000 spectrophotometer (Isogen Life Science, De Meern, The Netherlands).
(81) Enzyme Assays
(82) The initial total activity of GTFD enzyme of A. chroococcum NCIMB 8003 was determined by the amylose-iodine method (Bai et al., 2015b) using 0.125% (w/v) amylose V (AVEBE, Foxhol, The Netherlands) or 0.125% (w/v) potato starch (Sigma-Aldrich) as substrates. This assay measures the decrease in absorbance of the -glucan-iodine complex resulting from transglycosylation and/or hydrolytic activity. Enzymatic assays were performed with 28 g/ml of enzyme in 25 mM sodium phosphate buffer (pH 6.5) at 50 C. One unit of activity corresponds to the amount of enzyme converting 1 mg of substrate per min. The optimal pH and temperature were determined over the pH range of 4.5-9.5 and a temperature range of 30-75 C., using amylose V as substrate. Sodium acetate buffer (25 mM) was used at pH 4.5-6.0, MOPS buffer (25 mM) at pH 6.0-7.0, Tris-HCl buffer (25 mM) at pH 7.0-8.0, and glycine-NaOH at pH 9.0-9.5. For thermostability studies, the enzyme (0.5 mg/ml) was incubated in the absence of substrate for 10 min at different temperatures from 50 to 95 C., and then immediately cooled to 4 C. The residual activity was measured as described above.
(83) The initial activity of the purified P. beijingensis GTFD (PbGTFD) enzyme was determined using 0.125% (w v.sup.1) amylose V (AVEBE, Foxhol, The Netherlands) as substrate by the iodine-staining assay. This method monitors the decrease in absorbance at 660 nm in time of the -glucan-iodine complex resulting from transglycosylation and/or hydrolytic activity. Enzymatic assays were carried out with 12 g ml.sup.1 of enzyme in 25 mM sodium phosphate buffer (pH 7.0) containing 1 mM CaCal.sub.2 at 50 C. One unit of activity is defined as the amount of enzyme converting 1 mg of substrate per min. The optimal pH and temperature were determined over the pH range of 4.5-10.0 and a temperature range of 35-60 C. Sodium citrate buffer (25 mM) was used for pH between 4.5 and 7.0, Sodium phosphate buffer (25 mM) for pH between 7.0 and 8.0, Tris-HCl buffer (25 mM) for pH between 8.0 and 9.0, and sodium bicarbonate buffer for pH between 8.0 and 9.0.
(84) Substrate/Product Analysis with GTFD
(85) Purified GTFD enzyme (40 g ml.sup.1) of A. chroococcum NCBI 8003 was incubated separately with 25 mM sucrose (Acros), nigerose (Sigma-Aldrich), panose (Sigma-Aldrich), isomaltose (Sigma-Aldrich), isomaltotriose (Sigma-Aldrich), isomaltopentaose (Carbosynth), -cyclodextrins (Sigma-Aldrich), malto-oligosaccharides (MOS) with different degrees of polymerization (G2 to G7), and 0.6% (w/v) amylose V (AVEBE, Foxhol, The Netherlands), potato starch (Sigma-Aldrich) and amylopectin (Sigma-Aldrich). All reactions were performed in 25 mM sodium phosphate buffer, pH 6.5 with 1 mM CaCl.sub.2 at 37 C. for 24 h. The same conditions were used for the analysis of the oligosaccharides formed in time with maltohexaose and amylose V, but in this case 20 g ml.sup.1 of GTFD enzyme was used. For acceptor substrate studies, GTFD (40 g ml.sup.1) was incubated in 25 mM sodium phosphate buffer, pH 6.5, containing 1 mM CaCl.sub.2, with the acceptor substrates maltose or isomaltose (25 mM) in the presence of 0.35% (w/v) amylose V (donor substrate). The reaction mixtures were incubated at 37 C. for 24 h. In all cases, the progress of the reactions was followed by high-performance-anion-exchange chromatography (HPAEC) and/or thin-layer chromatography (TLC).
(86) The recombinant P. beijingensis GTFD enzyme (40 g ml.sup.1) was incubated separately with 25 mM sucrose (Acros), nigerose (Sigma-Aldrich), panose (Sigma-Aldrich), isomaltose (Sigma-Aldrich), isomaltotriose (Sigma-Aldrich), isomaltopentaose (Carbosynth), malto-oligosaccharides (MOS) with degrees of polymerization (DP) 2-7, and 0.6% (w/v) amylose V (AVEBE, Foxhol, The Netherlands), and amylopectin (Sigma-Aldrich). All incubations were performed in 25 mM sodium phosphate buffer (pH 7.0) with 1 mM CaCl.sub.2 at 37 C. for 24 h. Reactions were stopped by heating the samples to 100 C. for 8 min. The progress of the reactions was assessed by thin-layer chromatography (TLC) and/or high-performance-anion-exchange chromatography (HPAEC).
(87) Thin Layer Chromatography and High Performance Anion Exchange Chromatography with Pulsed Amperometric Detection Analysis
(88) Samples were spotted in 1-cm lines on TLC sheets (Merck Silica Gel 60 F254, 2020 cm), and after drying, the plates were run for 6 h in n-butanol:acetic acid:water, 2:1:1, v/v. The bands were visualized with orcinol/sulfuric acid staining and compared with a simultaneous run of a mixture of glucose and MOS (DP2 to DP7).
(89) Product mixtures from incubations with GTFD were analyzed by HPAEC on an ICS-3000 workstation (Dionex, Amsterdam, The Netherlands), equipped with an ICS-3000 ED pulsed amperometric detection system (PAD). The oligosaccharides were separated on a CarboPac PA-1 column (Dionex; 2504 mm) by using a linear gradient of 10-240 mM sodium acetate in 100 mM NaOH at a 1 ml/min flow rate. The identity of the peaks was assigned using commercial oligosaccharide standards.
(90) Production and Analysis of the Products from Amylose Incubation with GTFD
(91) Purified A. chroococcum and P. beijingensis GTFD enzymes (0.2 mg) were separately incubated with amylose V under the conditions described in Substrate/product analysis with GTFD. After incubation for 24 h at 37 C., the reactions were stopped by transfer to 95 C. for 6 min. The HMM polymer produced by the A. chroococcum GTFD enzyme was isolated by size-exclusion chromatography on a Bio-Gel P-2 column (2.550 cm; Bio-Rad) using 10 mM NH.sub.4HCO.sub.3 as eluent at a flow rate of 48 ml/h. The HMM and LMM polysaccharide fractions generated by P. beijingensis GTFD activity on amylose by size-exclusion chromatography on a Superdex S-200 (10300 mm; GE-Healthcare) using 25 mM ammonium bicarbonate as eluent at a flow rate of 0.5 ml min-1.
(92) (i) Methylation Analysis
(93) Methylation analysis of the isolated polysaccharides was performed as described before (van Leeuwen et al., 2008b) by per-methylation of the polysaccharides using CH.sub.3I and solid NaOH in DMSO, followed by acid hydrolysis with TFA. Partially methylated monosaccharides were reduced with NaBD.sub.4. The resulting partially methylated alditols were per-acetylated using pyridine:acetic anhydride (1:1 v/v) at 120 C. Partially-methylated alditol acetates (PMAAs) were analysed by GLC-EI-MS and GLC-FID as described (Van Leeuwen et al., 2008b).
(94) (ii) HPSEC Analysis
(95) The molecular mass distribution of the products mixtures were determined by HPSEC-MALS-RI as described previously (Bai et al., 2015b). Briefly, samples were dissolved at a concentration of 3.5 mg ml.sup.1 in DMSO-LiBr (0.05 M) and analyzed by high-performance size-exclusion chromatography coupled on-line with a multi angle laser light scattering detector (SLD 7000 PSS, Mainz), a viscometer (ETA-2010 PSS, Mainz) and a differential refractive index detector (G1362A 1260 RID Agilent Technologies). The separation was done by three PFG-SEC columns with porosities of 100, 300 and 4000 , coupled with a PFG guard column using DMSO-LiBr (0.05 M) as eluent at a flow rate of 0.5 ml min.sup.1. The system was calibrated and validated using a standard pullulan kit (PSS, Mainz, Germany) with M.sub.w ranging from 342 to 805 000 Da. The multiangle laser light scattering signal was used to determine the molecular masses of the amylose and the HMM polymers generated by the A. chroococcum and P. beijingensis GTFD enzymes with a refractive index increment value (dn/dc) of 0.072. The molecular mass of the P. beijingensis LMM polymer was determined by universal calibration method. WinGPC Unity software (PSS, Mainz) was used for data processing. Measurements were performed in duplicate.
(96) (iii) NMR Spectroscopy
(97) One-dimensional .sup.1H nuclear magnetic resonance (NMR) spectra of the product mixtures and the isolated polysaccharide were recorded in D.sub.2O on a Varian Inova 500 spectrometer (NMR Center, University of Groningen) at a probe temperature of 298K and processed with MestReNova 5.3 (Mestrelabs Research SL, Santiago de Compostella, Spain). Samples were exchanged twice in D.sub.2O (99.9 atom % D, Cambridge Isotope Laboratories, Inc., Andover, Mass.) with intermediate lyophilization, and then dissolved in 0.6 mL of D.sub.2O. Chemical shifts were expressed in ppm and calibrated by internal standard acetone ( 2.225 ppm). The percentage of different linkages was estimated by integration of the respective signal peak areas.
(98) Enzymatic Treatment of GTFD Product
(99) Reuteran GTFA polymer, IMMP GTFB polymer, P. beijingensis GTFD HMM and LMM polysaccharides and A. chroococcum GTFD polymer (5 mg/ml) were subjected to enzymatic digestions using excess -amylase (Aspergillus oryzae -amylase; Megazyme), dextranase (Chaetomium erraticum; Sigma-Aldrich), or pullulanase M1 (Klebsiella planticola; Megazyme). Enzymatic hydrolysis of each polymer was carried out in 50 mM sodium acetate buffer pH 5.0 for 48 h at 37 C. The degree of hydrolysis was analyzed by TLC and/or HPAEC analysis. Starch, dextran and pullulan, were used as positive controls for the -amylase, dextranase and pullulan treatments, respectively, resulting in complete hydrolysis under these conditions.
(100) Results and Discussion
Example 1: Identification of a Novel GH70 Protein Encoded by Azotobacter chroococcum
(101) Recently the identification of a novel GH70 subfamily represented by the Exiguobacterium sibiricum 255-15 GTFC 4,6--GT (designated GTFC enzyme) has been reported (Gangoiti et al., 2015). Aiming to find new enzymes active on maltodextrins and/or starch, but displaying different product specificities, a BLASTp search was carried out using the E. sibiricum GTFC protein as query sequence. As described before (Gangoiti et al., 2015), this allows identification of GTFC homologs in various Exiguobacterium and Bacillus strains, sharing more than 75 and 54% of identity with the E. sibiricum GTFC protein, respectively (Table 2). This new BLASTp search also resulted in identification of an additional GTFC homolog (78% coverage, 39% identity with the E. sibiricum GTFC) present in the recently elucidated genome of Azotobacter chroococcum NCIMB 8003 (ATCC 4412), annotated as a dextransucrase (Robson et al., 2015). The next hits obtained using BLASTp were (putative) GTFB-like 4,6--glucanotransferases followed by (putative) family GH70 glucansucrases and family GH13 proteins. The evolutionary relationships among representative GH70 and GH13 family members identified by BLASTp are depicted in
(102) TABLE-US-00003 TABLE 2 GTFC- and GTFB-like sequences identified via a BLASTp search using the Exiguobacterium sibiricum 255-15 GTFC protein as query. GTFC-like sequences are indicated. Azotobacter chroococcum NCIMB 8003 GTFD enzyme is shown in bold. GTFC- NCBI protein names Organism Coverage Identity Length Accession like? Dextransucrase Exiguobacterium sibiricum 255-15 100% 100% 893 WP_012371512.1 Yes Dextransucrase Exiguobacterium undae DSM 14481 100% 94% 893 WP_028105602.1 Yes Dextransucrase Exiguobacterium antarcticum B7 100% 93% 893 WP_014971370.1 Yes Dextransucrase Exiguobacterium antarcticum DSM 14480 100% 93% 893 WP_026830256.1 Yes Dextransucrase Exiguobacterium sibiricum 7-3 100% 92% 893 WP_026827371.1 Yes Dextransucrase Exiguobacterium acetylicum DSM 20416 100% 80% 892 WP_029342707.1 Yes Dextransucrase Exiguobacterium sp. RIT341 100% 75% 892 WP_035410561.1 Yes Dextransucrase Bacillus kribbensis DSM 17871 98% 56% 904 WP_035322188.1 Yes Dextransucrase Bacillus coagulans XZL4 81% 58% 755 WP_035317646.1 Yes Dextransucrase Bacillus coagulans H-1 79% 59% 730 WP_042872287.1 Yes Dextransucrase Bacillus coagulans 2-6 86% 55% 954 AEH52441.1 Yes alpha amylase, catalytic Bacillus coagulans DSM 1 = ATCC 7050 86% 54% 965 AJH79253.1 Yes domain protein Dextransucrase NCIMB 8003 78% 39% 780 AJE22990.1 Dextransucrase Lactobacillus fermentum ATCC 14931 72% 35% 1014 WP_003683900.1 Dextransucrase Lactobacillus fermentum 72% 35% 1478 WP_046948074.1 Dextransucrase Lactobacillus fermentum 28-3-CHN 72% 35% 986 WP_004563243.1 dextransucrase, partial Lactobacillus delbrueckii subsp. 71% 34% 966 EOD02243.1 jakobsenii ZN7a-9 = DSM 26046 glycosyl hydrolase family 70 Pediococcus pentosaceus IE-3 71% 34% 989 WP_036673144.1 glycosyl hydrolase family 70 Lactobacillus delbrueckii subsp. 71% 34% 954 WP_035171046.1 lactis CRL581 glycosyl hydrolase family 70 Lactobacillus delbrueckii subsp. 71% 34% 922 WP_044880492.1 delbrueckii DSM 20074 = JCM 1012 cell wall binding repeat Lactobacillus delbrueckii subsp. 71% 34% 957 WP_003613937.1 protein bulgaricus PB2003/044-T3-4 glycosyl hydrolase family 70 Lactobacillus delbrueckii subsp. 71% 34% 1210 WP_035182758.1 lactis DSM 20072 Dextransucrase Lactobacillus delbrueckii subsp. 71% 34% 1294 ADQ61508.1 bulgaricus ND02 putative glucansucrase Lactobacillus reuteri 78% 30% 1620 AAU08003.2 hypothetical protein Lactobacillus reuteri 78% 30% 885 WP_042746090.1 hypothetical protein Lactobacillus acidipiscis KCTC 13900 70% 35% 908 WP_035631372.1 putative glucansucrase Lactobacillus reuteri 78% 29% 1383 ABP88725.1 Dextransucrase Lactobacillus sanfranciscensis TMW 1.1304 64% 34% 866 WP_041818260.1 inactive glucansucrase Lactobacillus reuteri 121 80% 29% 1619 AAU08014.2 hypothetical protein Lactobacillus plantarum 74% 34% 1136 WP_045353679.1 hypothetical protein Lactobacillus plantarum 16 77% 29% 1414 WP_041161886.1 inactive glucansucrase Lactobacillus salivarius GJ-24 68% 34% 1626 EGM52218.1 Dextransucrase Lactobacillus reuteri DSM 20016 75% 30% 1363 ABQ83597.1 Dextransucrase Lactobacillus reuteri JCM 1112 75% 30% 1488 WP_003668618.1 Dextransucrase Lactobacillus reuteri mlc3 75% 29% 1488 WP_019251413.1
(103) This putative dextransucrase sequence of A. chroococcum is classified within family GH70 in the Carbohydrate-Active Enzymes (CAZy) database. Up to date, all GH70 members were encoded by members of the low GC phyla of Firmicutes, Gram-positive bacteria belonging exclusively to the orders Lactobacillales (GSs and GTFB-like 4,6--GTs) and Bacillales (GTFC-like 4,6--GTs). A. chroococcum NCIMB 8003 is an aerobic free-living member of the gamma-proteobacteria with the capacity to form dessication-resistant cysts. This Gram-negative bacterium is considered a model microorganism in the study of nitrogen fixation and hydrogen metabolism (Robson et al., 1984; Robson 1986). A. chroococcum has been recognized as a producer of extracellular exopolysaccharides (Lawson & Stacey, 1954; Cote & Krull, 1988). In view of its origin and its low sequence identity with other family GH70 proteins, we decided to carry out a detailed characterization of this novel enzyme and designated it as GTFD.
(104) A. chroococcum GTFD Protein Primary Sequence Analysis
(105) The complete amino acid sequence of GTFD from A. chroococcum encodes a polypeptide of 780 amino acids. This protein harbors a conserved Gram-negative signal peptide with a predicted signal peptidase cleavage site between amino acids 28 and 29, consistent with an extracellular location of this enzyme. Analysis of this GTFD sequence using the Pfam server revealed that two segments of the sequence (residues 82-255 and residues 416-780) are associated with family GH70. Sequence comparisons with E. sibiricum GTFC and L. reuteri GTFB revealed that A. chroococcum GTFD has the (non-permuted) domain organization observed for the E. sibiricum GTFC-like enzymes, and differs from GTFB and glucansucrases by a circular permutation of conserved regions I-IV. Thus, from the N-terminus to the C-terminus the A. chroococcum GTFD polypeptide chain successively contributes to domains An, Bn, IV, Bc, Ac and C, completely lacking domain V (
(106) Purification and Biochemical Properties of the A. chroococcum GTFD
(107) The gene encoding A. chroococcum GTFD enzyme without the putative signal sequence was cloned in-frame with an N-terminal His-tag and expressed in E. coli (DE3) BL21 star. Most of the GTFD protein was produced in soluble form and could be purified to homogeneity by metal-chelate chromatography (
(108) The effects of pH and temperature on A. chroococcum GTFD activity were determined using amylose V as substrate. The enzyme showed its maximum activity at 60 C. and at pH 6.5 and retained more than 70% of this activity over a pH range from 5.5 to 7.0 (
(109) Substrate and Product Specificity of the Azotobacter chroococcum GTFD
(110) The substrate specificity of GTFD was studied by incubating the enzyme with different oligosaccharides and polysaccharides at 37 C. for 24 h. The enzyme was inactive on sucrose, panose, nigerose, -cyclodextrins, and isomalto-oligosaccharides with DP2, DP3, and DP5. However, GTFD showed clear hydrolase/transglycosylase activity with malto-oligosaccharides (MOS) of DP3 to DP7 and formed a range of shorter and longer oligosaccharides (
(111) .sup.1H NMR analysis of the product mixture obtained with GTFD using amylose V and starch as substrates showed two broad signals in the anomeric region (=5.40-5.35 and 4.97) corresponding to the (1.fwdarw.4) and the newly synthesized (1.fwdarw.6) linkages (
(112) The molecular mass distribution of the products generated by GTFD from amylose V was determined by HPSEC-MALS-RI analysis (
(113) Characterization of the Polymer Synthesized by the A. chroococcum GTFD from Amylose V
(114) For further analysis the amylose V derived high molecular mass polymer was isolated by size-exclusion chromatography on Biogel P-2 column by collecting the void-volume fraction. 1D .sup.1H NMR analysis of this polymer revealed that 68 and 32% of the glucosyl units are forming (1.fwdarw.4) and (1.fwdarw.6) linkages, respectively, indicating a slight increase in the percentage of (1.fwdarw.6) linked glucose residues over those in the reaction mixture. The .sup.1H NMR spectrum of this GTFD polymer (
(115) TABLE-US-00004 TABLE 3 Structural analysis of the polymer produced by Azotobacter chroococcum NCIMB 8003 GTFD enzyme from amylose V. Type of glucosyl A. chroococcum L. reuteri 121 Parameter units GTFD polymer GTFA reuteran.sup.c Methylation Glcp(1.fwdarw. 19 7 analysis(%) .fwdarw.4)-Glcp-(1.fwdarw. 45 47 .fwdarw.6)-Glcp-(1.fwdarw. 18 35 .fwdarw.4,6)-Glcp-(1.fwdarw. 18 11 NMR chemical (1.fwdarw.4) 68 43 shift (%).sup.a (1.fwdarw.6) 32 57 Molecular mass 13 45 (10.sup.6 Da).sup.b .sup.aThe data represent the ratios of integration of the surface areas of the (1.fwdarw.6) linkage signal at 4.97 ppm and the (1.fwdarw.4) linkage signal at 5.36 ppm in the .sup.1H NMR spectra of the polysaccharides (see FIG. 4). .sup.bThe average molecular mass of polysaccharide was determined in duplicate. .sup.cTaken from Kralj et al., 2005.
(116) Oligosaccharides Formed in Time from Maltohexaose and Amylose V by the A. chroococcum GTFD Enzyme
(117) In order to get information about the formation of products in the progress of time, both maltohexaose and amylose V were incubated with GTFD, and samples for HPAEC analysis were taken at different time points (
(118) A. chroococcum GTFD Acceptor Substrate Reaction Studies
(119) To gain a better understanding of the mode of action of the A. chroococcum GTFD, the acceptor substrate specificity of this enzyme was studied and compared to that of L. reuteri GTFB (
(120) These results indicate that GTFD and GTFB have the ability to synthesize (1.fwdarw.4) linkages and (1.fwdarw.6) linkages when an acceptor substrate of low DP such as maltose is present. Isomaltose was a poor acceptor substrate for GTFD. HPAEC analysis showed that in the presence of isomaltose, GTFD does not form large amounts of oligosaccharides, and only small amounts of maltose and an unknown product were identified (
(121) Enzymatic Hydrolysis of the A. chroococcum GTFD Polymer
(122) To further explore the nature of the A. chroococcum GTFD polymer and to compare it with the polymers synthesized by L. reuteri 121 GTFA GS (reuteran) and GTFB 4,6--GT (IMMP), these 3 -glucans were treated with a high-dose of -amylase, dextranase and pullulanase enzymes (
Example 2: In Vitro Digestibility of Gelatinized Wheat Starch Treated with A. chroococcum GTFD
(123) Generation of the A. chroococcum GTFD -glucan from wheat starch
(124) A 0.6% suspension was prepared with wheat starch (Sigma S5127) in water. The suspension was heated to 90 C. for 10 min to gelatinize the starch and subsequently cooled to 37 C. Three hundred and thirty three L of 50 mM CaCl.sub.2 solution were added to the gelatinized starch suspension followed by 283 L of A. chroococcum GTFD (AcGTFD) enzyme solution (667 g of enzyme/100 mg starch). Starch suspension was incubated for 24 h at 37 C. After incubation, the treated suspension was heated at 95 C. for 6 min to inactivate the AcGTFD enzyme. Finally, the treated starch suspension was freeze-dried to obtain a powder of the AcGTFD generated material.
(125) Preparation of Digestive Enzymes for Assay
(126) Pancreatin from porcine pancreas (Sigma P7545) and intestinal acetone powders from rat (Sigma 11630) were extracted in 10 mM PBS solution (pH 6.8) at a 40 mg enzyme powders per mL concentration. Enzyme suspensions were vortex-mixed and sonicated in iced water for 7 min. Sonicated suspensions were then centrifuged at 10,000g for 30 min at 4 C. Supernatants were collected and protein content as well as enzyme activities were measured.
(127) Protein Content Measurements in Digestive Enzyme Preparations
(128) Protein was quantified in the supernatants obtained from the enzyme extractions with the BCA (Bicinchoninic Acid) kit for protein determination (Sigma BCA1-1KT). Supernatants were diluted 10 times and protein contents were measured after reacting with BCA reagent for 30 min at 37 C. in a spectrophotometer at 562 nm wavelength. A standard curve was prepared with bovine serum albumin standards for the calculation of total protein content.
(129) Measurements of Activity of Digestive Enzymes
(130) A 1% solution of soluble starch from potato (Sigma S2004) was prepared in 10 mM PBS solution (pH 6.8). One hundred microliters of 1% soluble starch solution were added to 100 l of pancreatin supernatant or rat intestinal acetone powders supernatant. Starch and enzyme mixtures were incubated at 37 C. for 10 min with constant stirring. Mixtures were subsequently boiled for 10 min to stop the enzymatic reaction. After allowing the mixtures to cool down, sample tubes were centrifuged at 10,000g for 10 min and glucose was measured via a colorimetric assay with the use of the Autokit Glucose (439-90901, Wako Diagnostics). One unit of enzyme activity was defined as the amount of protein required to hydrolyze 1 g of glucose from soluble starch.
(131) In Vitro Digestibility Measurements
(132) A 1% solution of the AcGTFD generated material was prepared in 10 mM PBS (pH 6.8). A 300 l aliquot of the solution was pre-heated to 37 C., along with the enzyme solutions, for 5 min. One hundred units/mg of the AcGTFD product of each digestive enzyme were added to the sample, standard and blank tube, in triplicate. Sample tubes were vortex-mixed and incubated for 20, 60, and 120 min at 37 C. with constant stirring. After each time point, a 0.5 mL aliquot of sample was transferred into a tube containing 1.5 mL of 90% aqueous ethanol. Sample aliquots in ethanol were stored at 4 C. until ready for glucose quantification. Sample aliquots were centrifuged at 10,000g for 10 min and glucose was measured via a colorimetric assay with the use of the Autokit Glucose (439-90901, Wako Diagnostics). 1. Results
(133) Treatment of gelatinized wheat starch with AcGTFD resulted in a material with a significantly lower rate and extent of in vitro digestibility. As can be observed from
Example 3: Identification of a Novel GH70 Protein Encoded by Paenibacillus beijingensis
(134) A protein homologous to the A. chroococcum GTFD was identified in the genome of Paenibacillus beijingensis DSM 24997 by BLASTp searches within the NCBI and IMG-ER platforms. A. chroococcum GTFD showed 48% identity in amino acid sequence to a hypothetical GH70 enzyme encoded by Paenibacillus beijingensis DSM 24997 (Genbank accession WP_052702730.1).
(135) Primary Sequence Analysis of the P. beijingensis GTFD Enzyme
(136) The identified P. beijingensis GTFD protein sequence consists of 776 amino acids and contains a putative secretion signal peptidase cleavage site between amino acids 30 and 31, in accordance with the extracellular location of GH70 enzymes. The domain organization of the P. beijingensis GTFD resembles that of E. sibiricum GTFC and A. chroococcum GTFD enzymes, regarded as structurally evolutionary intermediates between GH13 and GH70 families (
(137) On the basis of sequence alignments the four conserved regions of clan GH-H were identified in P. beijingensis GTFD and compared with those corresponding to other GH70 proteins. In accordance with its non-permuted domain organization, the order of these four conserved regions in P. beijingensis GTFD and A. chroococcum GTFD is I-II-III-IV, instead of the permuted order II-III-IV-I characteristic of GH70 glucansucrases and GTFB-like 4,6--GTases. The seven amino acid residues that are fully conserved in motifs I to IV of all GH70 family members are also found in both GTFD-like proteins (
(138) Purification and Biochemical Properties of the P. beijingensis GTFD Enzyme
(139) Recombinant P. beijingensis GTFD without its peptide signal sequence (amino acids 31-776) was expressed in soluble form at high levels and purified to homogeneity from E. coli BL21 star (DE3) by His-tag affinity chromatography yielding 50 mg of pure protein per liter of culture. SDS-PAGE analysis of the pure enzyme revealed the appearance of a single 80-kDa protein band (
(140) Substrate and Product Specificity
(141) The substrate specificity of the P. beijingensis GTFD (
(142) .sup.1HNMR analysis of the product mixture generated from amylose V revealed the presence of two broad anomeric signals corresponding to the (1.fwdarw.4) ( 5.40-5.35) and the newly formed (1.fwdarw.6) linkages (4.97) (
(143) Comparison of the products generated from amylose by the P. beijingensis and A. chroococcum GTFD enzymes by HPSEC with multi detection, revealed differences in their molecular mass distribution (
(144) Characterization of the High- and Low-Molecular Mass Polymers Produced by the P. beijingensis GTFD Enzyme from Amylose V
(145) For a more detailed characterization the HMM and LMM polymers generated from amylose V by the P. beijingensis GTFD were isolated by size-exclusion chromatography analysis on Sephadex S-200 and subjected to 1D/2D (1)H/(13)C NMR spectroscopy.
(146) TABLE-US-00005 TABLE 4 Structural characterization of the HMM and LMM polymers synthesized by the P. beijingensis GTFD enzyme from amylose V. P. beijingensis P. beijingensis Type of GTFD HMM GTFD LMM Parameter glucosyl units polymer polymer Methylation Glcp(1.fwdarw. 20 17 analysis (%) .fwdarw.4)-Glcp-(1.fwdarw. 45 54 .fwdarw.6)-Glcp-(1.fwdarw. 14 8 .fwdarw.4,6)-Glcp-(1.fwdarw. 21 21 NMR (1.fwdarw.4) 70 76 chemical (1.fwdarw.6) 30 23 shift (%).sup.a Molecular 27 10.sup.3 19 mass (10.sup.3 Da).sup.b .sup.aThe data represent the ratios of integration of the surface areas of the (1.fwdarw.6) linkage signal at 4.97 ppm and the (1.fwdarw.4) linkage signal at 5.36 ppm in the .sup.1H NMR spectra of the polysaccharides (see FIG. 4). .sup.bThe average molecular mass of polysaccharide was determined in duplicate.
(147) To gain more insight into the carbohydrate structures of the HMM and LMM P. beijingensis GTFD products, and to compare them with the A. chroococcum GTFD reuteran-like polymer and L. reuteri 121 GTFB IMMP, these -glucans were incubated for 48 h with different hydrolytic enzymes: -amylase, dextranase and pullulanase M1 (
(148) Composite Models.
(149) Using the data obtained by methylation analysis, NMR spectroscopy and enzymatic digestion studies composite models could be constructed, reflecting all major structural elements observed for the HMM and LMM P. beijingensis GTFD products (
(150) Oligosaccharides Formed in Time by the P. beijingensis GTFD Enzyme from Maltoheptaose
(151) To gain a better understanding of the reaction mechanism of the P. beijingensis and A. chroococcum GTFD enzymes, both enzymes were incubated with maltoheptaose (G7), and the oligosaccharides formed in time were analyzed by HPAEC (
Example 4: In Vitro Digestibility of Amylose Treated with A. chroococcum GTFD or P. beijingensis GTFD
(152) GTFD -glucans were generated as described above (see section Production and analysis of the products from amylose incubation with GTFD).
(153) Preparation of Digestive Enzymes for Assay
(154) Pancreatin from porcine pancreas (Sigma P7545) and intestinal acetone powders from rat (Sigma 11630) were extracted in 10 mM PBS solution (pH 6.8) at a 40 mg enzyme powders per mL concentration. Enzyme suspensions were vortex-mixed and sonicated in iced water for 7 min. Sonicated suspensions were then centrifuged at 10,000g for 30 min at 4 C. and supernatants were collected separately.
(155) Protein Content Measurements in Digestive Enzyme Preparations
(156) Protein was quantified in the supernatants obtained from the enzyme extractions with the BCA (Bicinchoninic Acid) kit for protein determination (Sigma BCA1-1KT). Supernatants were diluted 10 times and protein contents were measured after reacting with BCA reagent for 30 min at 37 C. in a spectrophotometer at 562 nm wavelength. A standard curve was prepared with bovine serum albumin standards for the calculation of total protein content.
(157) Measurements of Activity of Digestive Enzymes
(158) A 1% solution of soluble starch from potato (Sigma S2004) was prepared in 10 mM PBS solution (pH 6.8). One hundred microliters of 1% soluble starch solution were added to 100 l of pancreatin supernatant or rat intestinal acetone powders supernatant separately. Starch and enzyme mixtures were incubated at 37 C. for 10 min with constant stirring. Mixtures were subsequently heated at 100 C. for 10 min to stop the enzymatic reaction. After allowing the mixtures to cool down, sample tubes were centrifuged at 10,000g for 10 min and glucose was measured via a colorimetric assay with the use of the Autokit Glucose (439-90901, Wako Diagnostics). One unit of enzyme activity was defined as the amount of protein required to hydrolyze 1 g of glucose from soluble starch.
(159) In Vitro Digestibility Measurements
(160) 1% (w/v) solutions of PbGTFD-HMM, PbGTFD-LMM, AcGTFD-HMM, Amylose V, and gelatinized wheat starch were incubated with 100 units of porcine pancreatin and rat intestinal powder extracts in 10 mM PBS (pH 6.8) for 20, 60, and 120 min at 37 C. with constant stirring in a total volume of 1.15 ml. After each time point, samples were subsequently heated at 100 C. for 10 min to stop the enzymatic reaction. After allowing the mixtures to cool down, sample tubes were centrifuged at 10,000g for 10 min and glucose was measured via a colorimetric assay with the use of the Autokit Glucose (439-90901, Wako Diagnostics).
(161) Results
(162) The in vitro digestibility of the -glucan products obtained from Amylose V incubation with PbGTFD and AcGTFD enzymes was considerably reduced in comparison to gelatinized wheat starch in both rate and extent of digestion. As can be observed from
(163) Overall Conclusions
(164) In this study we report the characterization of the GTFD enzyme of A. chroococcum NCIMB 8003, providing the first example of a family GH70 enzyme in a Gram-negative bacterium. Regarding its amino acid sequence and domain organization, this enzyme is closely related to the E. sibiricum 255-15 GTFC, the first characterized member of a recently identified novel GH70 subfamily found in non-lactic acid bacteria (Gangoiti et al., 2015). GTFC type of enzymes are considered evolutionary intermediates between families GH13 and GH70, displaying 4,6--glucanotransferase activity with malto-oligosaccharides and amylose/starch, as previously found for the GTFB type of enzymes of lactobacilli. The E. sibiricum GTFC enzyme activity results in synthesis of isomalto/malto-oligosaccharides which consist of linear (1.fwdarw.6)-glucan chains attached to the nonreducing ends of MOS or starch fragments. In contrast, the A. chroococcum GTFD enzyme is unable to synthesize consecutive (1.fwdarw.6) linkages and converts amylose V into an -glucan with alternating (1.fwdarw.4) and (1.fwdarw.6) glucosidic bonds, and with (1.fwdarw.4,6) branching points. The GTFD polymer produced from amylose V thus is more similar to the reuteran produced from sucrose by the L. reuteri GTFA glucansucrase (Kralj et al., 2004; van Leeuwen et al., 2008a; Dobruchowska et al., 2013).
(165) The A. chroococcum GTFD is the first enzyme reported so far able to synthesize a reuteran-like polymer from amylose and/or starch. This GTFD enzyme is different from other starch-converting enzymes such as the family GH13 and GH57 branching enzymes that only introduce (1.fwdarw.6) branching points (Grimaud et al., 2014; Palomo et al., 2011) or the family GH15 dextrin dextrinases that synthesize consecutive (1.fwdarw.6) linkages (Naessens et al., 2005). Functionally, the A. chroococcum GTFD also differed from L. reuteri 121 GTFB and E. sibiricum GTFC in its mechanism of polymerization as it preferentially transfers an oligosaccharide per reaction cycle, visible in
(166) The A. chroococcum GTFD enzyme represents a powerful tool for the conversion of the starch present in food matrices into a health promoting food ingredient. Indeed, reuteran has been described as a potentially valuable food ingredient being regarded as a dietary fiber. Due to its highly branched structure, reuteran resists enzymatic degradation in the upper gastrointestinal tract and ends up in the large intestine where it can be fully fermented by the colonic microflora. In addition, it appears that reuteran enhances satiety in humans or animals (Ekhart et al., 2006), and can be used as a bread improver (Plijter et al., 2009). The in vivo role of this A. chroococcum GTFD reuteran-like polymer is unknown. It has been proposed that EPS provides protection to cells against desiccation and predation by protozoans or phage attack (Flemming & Wingender, 2010). Early studies reported that A. chroococcum strains NCIMB 8003 and NRRL B-14341 produce at least two exocellular polysaccharides, one which resembles alginate and a heteropolysaccharide (Lawson & Stacey, 1954; Cote et al., 1988). Following growth of A. chroococcum NRRL B-14341 on starch the same exopolysaccharides were isolated (Cote et al., 1988). Studies in A. vinelandii have demonstrated that alginates are essential for cyst formation (Nunez et al., 1999), and play a role in the protection of the O.sub.2-sensitive nitrogenase responsible of nitrogen fixation (Sabra et al., 2000). The A. chroococcum GTFD may have a related physiological function.
(167) We also report on the characterization of the GTFD enzyme of P. beijingensis DSM 24997, a further enzyme able to synthesize a reuteran-like polymer from amylose and/or starch. Whereas the A. chroococcum GTFD activity on amylose results in the synthesis of a high molecular polymer, in addition to maltose and other small oligosaccharides, two reuteran-like polymer distributions are produced by P. beijingensis GTFD: a high-molecular mass polymer with an average Mw of 27 MDa and a low-molecular mass polymer with an average Mw of 19000 Da. Besides, P. beijingensis GTFD is able to transfer longer MOS units than the A. chroooccum counterpart yielding reuteran polymers containing longer linear (1.fwdarw.4) sequences. From in vitro digestibility studies, all these polymers show a lower digestibility by digestive enzymes, providing strong support for the application of these enzymes for the reduction of glycemic Index of starchy products.
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