Transglycosylation by a chitinase from Enterobacter cloacae subsp. cloacae generates longer chitin oligosaccharides

Humans have exploited natural resources for a variety of applications. Chitin and its derivative chitin oligosaccharides (CHOS) have potential biomedical and agricultural applications. Availability of CHOS with the desired length has been a major limitation in the optimum use of such natural resources. Here, we report a single domain hyper-transglycosylating chitinase, which generates longer CHOS, from Enterobacter cloacae subsp. cloacae 13047 (EcChi1). EcChi1 was optimally active at pH 5.0 and 40 °C with a Km of 15.2 mg ml−1, and k cat/Km of 0.011× 102 mg−1 ml min−1 on colloidal chitin. The profile of the hydrolytic products, major product being chitobiose, released from CHOS indicated that EcChi1 was an endo-acting enzyme. Transglycosylation (TG) by EcChi1 on trimeric to hexameric CHOS resulted in the formation of longer CHOS for a prolonged duration. EcChi1 showed both chitobiase and TG activities, in addition to hydrolytic activity. The TG by EcChi1 was dependent, to some extent, on the length of the CHOS substrate and concentration of the enzyme. Homology modeling and docking with CHOS suggested that EcChi1 has a deep substrate-binding groove lined with aromatic amino acids, which is a characteristic feature of a processive enzyme.

Enterobacter cloacae subsp. cloacae (Ec), a nosocomial pathogen, was originally isolated from the human cerebrospinal fluid by Edwin Oakes Jordan in 1890 16 . Analysis of the genome sequence of E. cloacae subsp. cloacae revealed that four chitinases and two N-acetyl-glucosaminidases could be involved in chitin degradation. In addition, E. cloacae genome has genes that code for one CBM-33 lytic polysaccharide monooxygenase (LPMO-GenBank: ADF60226.1) and one polysaccharide deacetylase (PDA-GenBank: ADF62202.1), which may have a crucial role in depolymerization of chitin. Of the four chitinases, two belong to family GH18 (EcChi1-GenBank: ADF62010.1 and EcChi2 (GenBank: ADF62328.1) and other two belong to GH19 (EcChi3-GenBank: ADF62326.1 and EcChi4-GenBank: ADF61237.1). Here, the EcChi1 with only the catalytic GH18 domain and no auxiliary domains displayed an unprecedented hyper-TG. We show that EcChi1 has structural features of a hyper-TG chitinase similar to SpChiD of Serratia proteamaculans.

Results
Cloning, heterologous expression, purification and dot blot assay. Full-length DNA sequence coding for EcChi1 consisted of 1257 nucleotides and an ORF of 418 amino acid residues with a predicted isoelectric point of 6.15. A 1.2-kb segment of EcChi1 gene was amplified with specific primers using gDNA of E. cloacae subsp. cloacae as a template, cloned into pET-28a (+), and transformed E. coli Rosetta-gami for expression. Extracellular protein was isolated from the induced E. coli Rosetta-gami culture pellet and purified EcChi1 through Ni-NTA affinity chromatography. The molecular mass of EcChi1 (42.5 kDa) calculated from amino acid sequence without the signal peptide was in agreement with experimentally observed molecular weight as obtained by 12% SDS-PAGE ( Supplementary Fig. S1A). Dot -blot assay revealed that, EcChi1 exhibited clear zone on water-soluble glycol chitin containing gel confirming the chitinase activity ( Supplementary Fig. S1B).
Steady state kinetics of EcChi1 on colloidal chitin and chitobiose. The EcChi1 was active in mildly acidic to a neutral range of pH 5.0 to 7.0 with the optimum activity in 50 mM sodium citrate pH 5.0 (Fig. 1A). However, the activity decreased sharply below pH 5.0 and above 7.0, with diminished or no activity below pH 4.0 and above 9.0. EcChi1 was optimally active at 40 °C (Fig. 1B) and retained 60% activity at 50 °C, that was decreased with increase of temp up to 80 °C, while 70% activity was retained at 30 °C. The effect of metal ions on the activity of EcChi1 was also evaluated using colloidal chitin as substrate. The activity of EcChi1 in presence of Cu +2 was similar to control but was partially inhibited in the presence of urea, Ca +2 , Mg +2 , Zn +2 , Mn +2 , EDTA, and Fe +2 . The presence of Hg +2 and SDS inhibited the activity by 80% and 90%, respectively. There was no increase in the activity of EcChi1 in the presence of test cations. The kinetic parameters of EcChi1 were determined with colloidal chitin and chitobiose as the substrate. The velocity measurements fitted to Michaelis-Menten kinetics revealed that the K m , k cat , and k cat /K m values were 15.2 mg ml −1 , 0.16 × 10 2 min −1 and 0.011 × 10 2 mg −1 ml min −1 for colloidal chitin (Fig. 1C) and 213.2 μM, 1.41 min −1 and 0.6 × 10 −2 for chitobiose ( Supplementary Fig. S2).
Binding study with soluble substrates. Binding of EcChi1 to the soluble substrates was analysed using native PAGE with or without polysaccharides embedded in the gel. In presence of laminarin, CM-cellulose and glycol chitin there was a decrease in electrophoretic mobility of EcChi1 (Fig. 2). Among the three soluble substrates, the retardation in the mobility of EcChi1 was more by soluble glycol chitin than CM-cellulose, and laminarin suggesting specificity of EcChi1 towards chitinous substrates.
Time-course of colloidal chitin and oligosaccharide degradation. EcChi1 released DP1 to DP4 hydrolytic products on polymeric colloidal chitin substrate with DP2 and DP1 as the major products ( Fig. 3A and B). The concentration of DP1 increased with the extension of incubation time. EcChi1 hydrolyzed DP2 into DP1 after 240 min, and complete hydrolysis occurred by 420 min (Supplementary Fig. S3). Chitobiose was the major hydrolytic product from both DP3 and DP4 substrate ( Fig. 4A and B). With DP5 substrate, a very little DP1 (1.4%) formed from 120 min. After prolonged incubation, DP1 was the dominant product with 37.5% followed by DP2 with 28% at 720 min ( Fig. 5A and C). The hydrolysis of DP6 by EcChi1 was rapid with only 2.2% of DP6 at 120 min ( Fig. 5B and D).
Reaction with DP4 substrate accumulated TG products from 1 min and lasted for 480 min, while DP8 product was detectable until 240 min. The TG products DP5 and DP6 reached a maximum quantity of 5.3% and 4.4% at 60   The topmost profile shows a standard mixture of CHOS ranging from DP1 to DP6. The remaining profiles are the reactions at different incubation times. Control represents the substrate without EcChi1 while standard represents CHOS ranging from DP1 to DP6. (B) Overview of the quantifiable CHOS products generated during hydrolysis. Products were quantified from respective peak areas using standard calibration curves of CHOS ranging from DP1 to DP4. The other profiles show the reaction products from DP3 and DP4 substrates at the indicated incubation times. The inset shows a magnified view of the low-peak-area products. Control represents the substrate without EcChi1. Overview of concentrations of CHOS products generated during reaction time courses with DP3 (C) and DP4 (D) substrates. Products were quantified from respective peak areas using standard calibration curves of CHOS ranging from DP1 to DP6.
Scientific RepoRts | 7: 5113 | DOI:10.1038/s41598-017-05140-3 and 5 min, respectively ( Fig. 4B and D). With DP5 substrate, DP6-DP9 products formed due to TG. DP6 formed from 1 min that reached to a maximum (2.5%) by 45 min, that was hydrolyzed to shorter CHOS ( Fig. 5A and C). The CHOS DP7-DP9 were detectable TG products with DP6 substrate (Fig. 5B and D). The TG products formed from 1 min onwards and remained until 240 min.  The hydrolytic and TG activity of EcChi1 were assayed at low substrate and enzyme concentrations with DP4 substrate. EcChi1 exhibited remarkable TG activity even with the low substrate and enzyme concentrations. A 10-fold lower concentration of the substrate (100 μM) and enzyme (20 nM) resulted in the formation of DP5-DP7 as TG products until 30 min that was eventually degraded ( Supplementary Fig. S4A). When the substrate concentration decreased by 20 fold (50 μM), the TG products, DP5 and DP6 formed between 0-8 min, which gradually decreased over time ( Supplementary Fig. S4B). These results indicated that the TG activity of EcChi1 was proportional to the substrate concentration.
Docking of EcChi1 with chitin tetramer. Sequence analysis revealed that EcChi1 is a single modular GH18 chitinase. The closest homologue of EcChi1 with a known crystal structure was chitinase II from Klebsiella pneumoniae (PDB: 3QOK; 86% sequence identity) which was used as the template to generate a 3D model. The stereo chemical quality of the generated model was checked for its quality through Ramachandran plot generated from PROCHECK analysis. The model showed 92.1% amino acids of modelled protein fell in the most favored region. Verify-3D graph also showed that 95.71% of the residues had an averaged 3D-1D score > = 0.2. Coordinates for chitin tetramer were extracted from the crystal structure of chitinase A from Serratia marcescens (PDB: 1NH6) and docked with modelled EcChi1 protein. EcChi1 complexed with DP4 substrate showed binding of DP4 from +2 to −2 subsites. Trp114 and Tyr154 and Arg278 and Trp395 are present at +2, +1 and −1, −2 positions, respectively. The residues forming interactions with ligand in the protein-ligand complex were Trp114, Tyr154, Arg278, and Trp395. Amino group in indole ring of Trp395 formed the hydrogen bond with a distance of 3.5 Å with the oxygen of acetamido group of non-reducing sugar moiety and a hydroxyl group on C6 of non-reducing sugar the formed hydrogen bond with 2.8 Å distance with the carboxylic group of Trp114, at −2 subsite (Fig. 7B). A terminal guanidium amino group of Arg278 and the amino group of Trp114 formed a hydrogen bond with 3.4 Å and 2.1 Å distances with the hydroxyl group of C6 and C4 of the penultimate non-reducing sugar moiety, respectively at −1 subsite. The hydroxyl group of Tyr154 formed a hydrogen bond with the hydroxyl group on C6 of sugar moiety at +1 subsite with 1.9 Å distance (Fig. 7B). EcChi1 has deep substrate binding cleft lined with aromatic residues that may play a major role in TG activity. The two aromatic amino acids Trp114 and Trp395 are located near to the catalytic center Glu153 (Fig. 7A and C).

Discussion
The recent advances in whole genome sequencing technologies have paved the way to mine bacterial genomes for the genes and proteins of industrial importance. Search for new chitinases by utilizing the available genome information from diverse bacteria may provide chitinases with high TG activity for generating longer-chain CHOS. Phylogenetic analysis of chitinases from diverse bacterial members showed clustering of chitinases belonging to Enterobacteriaceae members along with a well characterized hyper-TG chitinase SpChiD with a few exceptions 17 . This observation suggested that mining Enterobacteriaceae members could be an option for novel TG enzyme. In the present study, we have identified and characterized a hyper-TG chitinase (EcChi1) from Enterobacter cloacae, a familiar representative species of family Enterobacteriaceae. Very few reports are available on chitinases and chitinolytic system of Enterobacter sp (Table 1). Among which, Enterobacter sp. G-1 18 , E. aerogenes 19 , and Enterobacter sp. NRG4 20 chitinases were characterized. ChiA was the first reported chitinase 21 from an Enterobacter sp and shared 26% sequence homology with EcChi1. EcChi1 exhibited 87% sequence similarity with E. aerogenes chitinase, which did not have TG activity. There is no correlation between overall sequence similarity and TG as it depends on active site architecture of the enzyme and the orientation of water molecules at the catalytic centre which favors binding of incoming carbohydrate molecules, through strong interactions in the aglycon subsites 22 . The amino acid sequence of EcChi1 showed 87% identity to that of GH18 chitinase II (PDB ID: 3QOK) from Klebsiella pneumoniae for which no characterization was available. EcChi1 shared 75% identity with a hyper-TG chitinase of S. proteamaculans (SpChiD) (PDB ID: 4NZC) 11 . Nevertheless, many chitinases showing TG such as ChiA1 from B. circulans WI-12 23 , ChiA from Vibrio harveyi 24 , and human chitotriosidase-1 25 showed only 31%, 26% and 29% sequence similarity to EcChi1, respectively.
Enzymes show a pH range at which they are most active. EcChi1 was optimally active at slightly acidic pH (pH 5.0-6.0) similar to the chitinases A, B, and D from S. proteamaculans 11,26 , chitinase B from S. marcescens 27 , Paenibacillus sp. D1 28 and Enterobacter sp. NRG4 29 . EcChi1 optimally active at 40 °C comparable to SpChiB, SpChiC 26 , SpChiD 11 and Chitinibacter sp. GC72 30 . The optimum temperature of EcChi1 was higher than many other chitinases such as Vibrio sp 31 and S. antarcticus 32 . However, some chitinases from B. cereus IO8 33 and Paenibacillus barengoltzii 34 exhibited high optimal temperature than EcChi1.
Unlike pH and temperature optima, the kinetic parameters of EcChi1 were different from SpChiD. The K m and catalytic efficiency (k cat /K m ) of EcChi1 were 6 fold decrease and nearly 2 fold increase than SpChiD, respectively 11 . Among all the kinetic parameters, there is a significant correlation between K m and TG, whereas no direct correlation between k cat and TG activity was observed in chitinases 35 . The single mutants of ChiA-D313N and ChiB-D142N from S. marcescens showed 2 to 3 fold lower K m and increased TG than the wild-type. The hydrophobicity of amino acids at substrate acceptor region and catalytic groove makes the enzyme efficiently bind to the substrates which resulted in less K m . The overall catalytic efficiency (k cat /K m ) of EcChi1 was lower than ChiA, ChiB and, ChiC from S. proteamaculans 26 possible attributed to the lack of accessory domain (s) in EcChi1. The activity of EcChi1 on crystalline α-chitin and β-chitin was also low in comparison to colloidal chitin due to lack of accessory domains. The lining of aromatic amino acids in a substrate binding groove of EcChi1 (Fig. 7A) might responsible towards chitinous polymeric substrates. Similar findings were observed for SpChiD and StmChiA but not for StmChiB 11,12 . EcChi1 had a very low activity on avicel (Fig. 1D). This could be due to the non-specific activity of EcChi1, as reported in a chitinase (ChiC) from Pseudoalteromonas sp. DL-6 36 . Various cations, particularly metal ions influence the activity of chitinases 37 . Certain ions such Cu +2 and Zn +2 act as either stimulators or inhibitors on chitinases 38 , not in the case of EcChi1.
The highly conserved catalytic motif (DxxDxDxE) and chitin-binding motif (SXGG) are positioned between 146-153 and 110-113 amino acids, respectively. Single amino acid residue present immediate to the chitin-binding motif and presence of α/β fold insertion plays a pivotal role in processivity 39 . The two aromatic amino acids Trp97 and Trp220 were crucial for processivity in ChiB from S. marcescens 40 . Presumably, corresponding aromatic amino acids Trp114 and Tyr226 might tightly bind with the polymeric substrate and steer the processive action of EcChi1, implying that EcChi1 might be a processive enzyme (Fig. 7A and C). In addition, homology modelling studies of EcChi1 showed the presence of deep substrate binding cleft lined with twelve aromatic amino acids, and α/β fold insertion further support the characteristic feature of a processive enzyme. Analysis of product profile for dominance of even number oligosaccharides and the ratio of DP2/DP1 have been employed to determine an apparent degree of processivity 41,42 . For example, the ratio of initial DP2/DP1 for two processive enzymes SmChiA and SmChiB had 30.1 ± 1.5 and 24.3 ± 2.0, respectively 42 . Upon degradation of colloidal chitin by EcChi1, DP1 was not detectable up to 60 min indicating a possible processive mode (Fig. 3B). At 90 min the DP2/DP1 ratio was 1.45, which further decreased with increase in time possible because of chitobiase activity of EcChi1.
HPLC analysis revealed that DP2 and DP1 are the major end products with colloidal chitin substrate similar to SpChiD and StmChiA 11,12 . Gradual formation of DP1 from DP2 indicated chitobiase activity and DP2 was not a suitable substrate for TG. EcChi1 exhibited marginally lower k cat when compared to SpChiD. The sequence analysis and modelling studies showed EcChi1 having a unique loop (Asn30 -Asp42) present at N-terminal region. The amino acids present at substrate binding cleft were occupied by the loop structure. The unique loop and aromatic residues highly conserved in single domain GH18 Enterobacteriaceae chitinases. The conserved amino acids Tyr28, Val35, and Thr36 might be responsible for chitobiase activity in EcChi1 similar to SpChiD 17 . TG is a far-flung phenomenon in GH18 family chitinases, little known about the structural basis underlying this integral activity. EcChi1 showed significant TG activity on CHOS and produced long chain CHOS up to DP9. The product profile with DP3 substrate suggested that −1 to +2 or −2 to +1 subsites are possible for productive binding. DP3 was the minimum length of the substrate for EcChi1 to show TG activity. DP1-DP8 products were detected with DP4 substrate in which DP5-DP8 were TG products, whereas DP5-DP9 were TG products in SpChiD 11 . DP9 was the longest TG product detected with both DP5 and DP6 substrates. Similarly, incubation of 5 mM chitopentaose (DP5) with recombinant human chitotriosidase (HCT) resulted in the formation of the DP1-DP9 25 . No TG activity was observed by StmChiA with DP5 substrate 12 . EcChi1 synthesized long-chain CHOS even with low concentrations of substrate and enzyme. Amino acid residues positioned at acceptor binding site are assumed to be crucial for TG activity 43 . The known chitinases with TG activity were occupied with aromatic amino acids at +n subsites. Phe396&Trp275 and Trp220&Trp97 were occupied by the position at +2 and +1 subsites of ChiA and ChiB from S. marcescens, respectively 44,45 . Similarly, Trp114, Tyr154 at +1, +2 subsites might help further in delivering efficient TG activity in EcChi1. In addition, Trp285 and Trp164 are occupying in +2 and +1 subsites of ChiA from B. circulans 46 . It was further supported by a non-processive endochitinase from S. marcescens, SmChiC2 which lacks TG activity and aromatic amino acids at +1, +2 subsites 39 . Thus bulk aromatic amino acids present at positive subsites and the lining of aromatic amino acids at substrate binding cleft might be increased the binding affinities for upcoming sugar acceptor molecule thereby promoted TG activity in EcChi1.
In addition to processivity, single amino acid residue, present next to this chitin-binding motif (SXGG), plays an important role in TG 47,48 . SXGG motif was extended with tryptophan in other well-known TG chitinases, viz., HCT 25 , B. circulans ChiA 46 , ChiA and ChiB from S. marcescens 49 and SpChiD in S. proteamaculans 11 . In non-TG and non-processive endo-chitinases, such as SmChiC2 and LlChi18A, this tryptophan was substituted with small amino acid alanine indicated its probable role in TG 47,50 . Trp114 was the corresponding amino acid in EcChi1 which may contribute to TG and processivity. In addition, the highly conserved novel loop was identified among the GH18 single catalytic domain chitinases from Enterobacteriaceae, showing their divergence from other groups 17 . This unique loop (Asn30 -Asp42) is present in EcChi1 may favor the interaction with the incoming substrate molecule.
The degree of endo-activity is best assessed as a probability of endo-mode initiation where concentrations of both insoluble reducing groups (endo-initiation) and reducing end groups (exo-initiation) upon substrate degradation are determined 51 . Hence, the observation of CHOS with DP higher than DP2 is indicative of EcChi1 having endo-activity as observed for SmChiC. Homology modelling based structural analysis also suggests that EcChi1 has structural features of an endo-acting enzyme with an apparent processive mode of action. EcChi1 was the first reported chitinase from Enterobacter sp with high TG. The capability to hydrolyze chitin with high TG activity suggests EcChi1 could be a suitable enzyme for industrial production of long chain CHOS, while it would also be of interest to know the possible physiological role of EcChi1.

Methods
Chemicals and enzymes. Genomic DNA of E. cloacae subsp. cloacae ATCC 13047 was used as a template to amplify the EcChi1 gene. The plasmid pET-28a (+) and E. coli Rosetta-gami II (DE3) (Novagen, Madison, USA) were used for heterologous expression. E. coli was grown in Luria bertani (LB) broth (1% peptone, 0.5% yeast extract, 1% NaCl) at 37 °C. The antibiotics kanamycin (50 µg ml −1 ) and chloramphenicol (25 µg ml −1 ) were added to the medium as required. Oligonucleotide primers were designed based on the DNA sequence available in the database and procured from Integrated DNA Technologies (Bangalore, India). Restriction enzymes, T4 DNA ligase, and Q5 DNA polymerase were from New England Biolabs (NEB). Isopropyl-β-D-thiogalactoside (IPTG), kanamycin and all other chemicals were purchased from Calbiochem, Merck (Darmstadt, Germany) or from Hi-Media Labs (Mumbai, India). The polymeric substrates α-chitin (extracted from shrimp shells), β-chitin (extracted from squid pen), and high molecular weight chitosan substrates of a fraction of acetylation (F A ) = 0.10% (Mahtani Chitosan Pvt. Ltd.) and F A = 25% (Sigma-Aldrich) were used for enzyme assay. Colloidal chitin and glycol chitin were prepared as described earlier 52 . CHOS with different DP were purchased from Seikagaku Corporation (Tokyo, Japan). Avicel was procured from Sigma-Aldrich (St. Louis, MO).
DNA manipulations and cloning of EcChi1. E. cloacae genomic DNA (gDNA) was isolated as described by 53 . A gradient PCR, with appropriate gene-specific forward primer: 5′-CTC CCA TGG GAC TGA TGT CCG TG-3′and reverse primer: 5′-GGC CTC GAG CTT CGC TAA CTG GTT-3′ was used to determine the suitable annealing temperature for maximum amplicon yield. The amplicon was purified using PCR cleanup kit (MACHEREY-NAGEL GmbH & Co., Germany) and cloned into the Nco I and Xho I sites of the pET-28a (+). The construct was used to transform E. coli Rosetta-gami-II (DE3) for expression of the cloned gene. Transformants were selected on kanamycin and chloramphenicol containing LB plates. The nucleotide sequence of the insert was confirmed by automated DNA sequencing (Scigenom, Kerala, India).
Expression and purification of EcChi1. Expression and purification of EcChi1 were done as described by ref. 52. The expressed protein was purified using Ni-nitrilotriacetic acid (Ni-NTA) affinity chromatography. Fractions of eluate having EcChi1were pooled and the protein purity was assessed by performing 12% SDS-PAGE. The purified EcChi1, in 50 mM sodium citrate buffer (pH 5.0), was stored at 4 °C for further characterization. The protein content of the sample was measured using a bicinchoninic acid (BCA) protein assay kit (Thermo Scientific, USA) where bovine serum albumin (BSA) as a standard.
A composite gel mixed with 0.1% glycol chitin was prepared. Five micrograms of EcChi1 was spotted onto the gel and placed in the humid chamber at 37 °C overnight. After incubation, the gel was stained with 0.01% calcofluor white M2R in 0.5 M Tris-HCl (pH 8.9) for 10 min at 28 ± 2 °C. Finally, the brightener solution was removed. The gel was washed three times with distilled water for every 10 min at 28 ± 2 °C. The lytic zone was visualized on a UV transilluminator.
Reducing end assay. Chitinase activity was measured by a reducing-end assay as described by ref. 54 with slight modifications. Recombinant EcChi1 was incubated with colloidal chitin in 50 mM sodium citrate pH 5.0 at 40 °C, 200 rpm for 1 h, followed by centrifugation at 13,600 × g, 4 °C for 30 min. A 40 μL of the clear supernatant containing reducing groups was mixed with 300 μL of the freshly prepared color reagent (0.5 M sodium carbonate, 0.05% potassium ferricyanide) and boiled for 15 min at 120 °C. Optical density was measured for 200 μL of each reaction mixture at 420 nm. One unit was defined as the amount of enzyme that liberated 1 μmol of reducing sugar per min. All the reactions were performed in triplicate.
Optimum pH and temperature. To determine the optimum pH, the purified EcChi1, and colloidal chi- Substrate specificity. The substrate specificity of the purified EcChi1 was determined by replacing the colloidal chitin in the reaction mixture with different insoluble chitinous and non-chitinous substrates viz., α-chitin, β-chitin, colloidal chitin, glycol chitin (water-soluble chitin), chitosans (F A = 0.1 and 25%), or Avicel (microcrystalline cellulose). EcChi1 (3.5 μM) was incubated with different substrates (2.5% wt/vol) at 40 °C for 1 h followed by reducing end assay. For each experiment, we individually calculated the reducing ends present in substrate alone and deducted the initial number of reducing groups from the value obtained from the enzyme-substrate reaction. One unit was defined as the amount of chitinase that liberated 1 μmol of reducing sugar per min.
Soluble substrate binding. Soluble substrate binding was assessed as described by ref. 52. Different soluble polymeric substrates, viz., glycol chitin, laminarin, and CM-cellulose were incorporated in 8% polyacrylamide gels. BSA was loaded as a non-interacting protein. The electrophoresis was performed at 4 °C at a constant voltage of 80 V. The gels were stained with coomassie blue G-250 to detect the proteins. Binding was assessed visually or alternatively, the migration distances of the chitinases and protein marker were measured directly on the resolving gels.

Effect of various additives.
To determine the effect of various additives viz., metal ions (Ca +2 , Cu +2 , Fe +2 , Mg +2 , Mn +2 , Hg +2 , Zn +2 ), chelator (EDTA) and denaturants (Urea, SDS), of 1 mM each were added to EcChi1 with colloidal chitin as a substrate. After a pre-incubation for 1 h at 40 °C at 200 rpm activity was measured by reducing end assay. For each additive, the residual activity was calculated, considering the activity without additive was 100%.

Time-course of colloidal chitin and oligosaccharide degradation. The hydrolytic activity of EcChi1
was assessed in a reaction mixture containing 1 mM substrate and 200 nM purified EcChi1 in 50 mM citrate buffer, (pH 5.0) at 40 °C over 720 min. The reaction was terminated by transferring 40 µL of the reaction mixture to an Eppendorf tube containing an equal amount of 70% acetonitrile and stored at −20 °C until analysis. Aliquots of 20 μL were injected into HPLC (Shimadzu, Tokyo, Japan) equipped with a ShodexAsahipack NH2P-504E column (4.6 mm [inner diameter] by 250 mm; Showa Denko K.K). Briefly, the mobile phase consisted of 70% acetonitrile and 30% MilliQ H 2 O, the flow rate was set to 0.7 ml min −1 . The eluted CHOS were monitored at 210 nm. A CHOS mixture containing equal weights of oligomers ranging from DP1 to DP6 was used to generate standard chromatogram. Calibration curves were constructed separately for each CHOS in the mixture. The data points generated a linear curve for each CHOS with r 2 values of 0.997 to 1.0.

MALDI-TOF MS analysis.
The products of the reaction mixture with DP5 and DP6 CHOS substrates were analyzed by matrix-assisted laser desorption ionization time of flight mass spectrometry (MALDI-TOF MS) after 45 min and 15 min, respectively. A 40 μL of the reaction mixture was concentrated and redissolved in 10 μL of HPLC-grade MilliQ H 2 O (Merck, Mumbai, India). Two microliters sample was mixed into the 2,5-dihydroxybenzoic acid (DHB) droplet and dried under a stream of air and analysis was done using Ultraflex MALDI-TOF/TOF (BrukerDaltonics GmbH, Bremen, Germany) with an autoflex 123 smart beam. The instrument was operated by the FlexControl 3.0 software package. All spectra were obtained using the reflectron mode with an acceleration voltage of 25 kV, a reflector voltage of 26, and pulsed ion extraction of 40 ns in the positive ion mode. The acquisition range was from m/z 800 to 2000. Peak lists were generated from the MS spectra using BrukerFlex Analysis software (version 3.0). Docking of EcChi1 with chitin tetramer. The protein sequence of EcChi1 was retrieved from NCBI Database (http://www.ncbi.nlm.nih.gov/) with accession number ADF62010.1 for modeling. To select appropriate templates for constructing 3D structure models of the EcChi1 protein, The BLAST program was used for sequence search against known 3D structure available in the Protein Databank (PDB) (http://www.rcsb.org/), The homology model program MODELLER v9.12 55 was employed to generate 3D models of EcChi1 based on the crystal coordinates of chitinase II from Klebsiella pneumoniae (PDB: 3QOK). The stereochemical quality of the modeled protein structure was checked in Ramachandran plot 56 using PROCHECK 57 . The compatibility of the model with its sequence was measured by Verify-3D graph 58,59 . Chitin tetramer ligand was extracted from the 1NH6 crystal structure, using Discovery studio 4.0 and used for docking studies using Autodock 4.2 60 via Auto Dock Tools (ADT) graphical user interface. Interactions with ligand were viewed in PyMol Molecular Graphics System 1.7.