Pectinolytic Bacterial Consortia Reduce Jute Retting Period and Improve Fibre Quality

Jute fibre is the second most important fibre next to cotton. It is obtained from the bark of plant through microbial retting process. Here we report optimized microbial retting protocol that can lower retting period and produce high fibre quality. A total of 451 bacterial colonies have been isolated from five jute retting water samples in Bangladesh. Higher pectinolytic bacterial isolates were predominant in the later stage of jute retting. Out of these, 168 isolates have been screened by both semi-quantitative and quantitative pectinase, xylanase and cellulase enzyme assay. Among them, 144 isolates have been selected on the basis of extra cellular enzyme activity of these three enzymes. 16 s ribosomal gene sequencing analysis identified 2 phyla- Firmicutis (80.55%) and Proteobacteria (19.45%). To check the synergistic and antagonistic effect 10 selected isolates were tested in 167 different combinations. Three best combinations were identified that lowered retting period from 18–21 days to 10 days producing high quality fibre in both laboratory and field trial. This improved retting technology can be adopted in industrial scale for the production of quality jute fibre in a controlled condition in reduced water quantity without polluting the environment.

Jute fibre is the second most important fibre next to cotton. It is obtained from the bark of plant through microbial retting process. Here we report optimized microbial retting protocol that can lower retting period and produce high fibre quality. A total of 451 bacterial colonies have been isolated from five jute retting water samples in Bangladesh. Higher pectinolytic bacterial isolates were predominant in the later stage of jute retting. Out of these, 168 isolates have been screened by both semi-quantitative and quantitative pectinase, xylanase and cellulase enzyme assay. Among them, 144 isolates have been selected on the basis of extra cellular enzyme activity of these three enzymes. 16 s ribosomal gene sequencing analysis identified 2 phyla-Firmicutis (80.55%) and Proteobacteria (19.45%). To check the synergistic and antagonistic effect 10 selected isolates were tested in 167 different combinations. Three best combinations were identified that lowered retting period from 18-21 days to 10 days producing high quality fibre in both laboratory and field trial. This improved retting technology can be adopted in industrial scale for the production of quality jute fibre in a controlled condition in reduced water quantity without polluting the environment.
Jute, second most important natural fibre after cotton, is cultivated in East Asia and some parts of Latin America 1-3 . Jute is a bast or phloem fibre in the bark of stems, cemented together by pectin and gummy substances 4 . Commercial extraction of jute fibre is water based microbiological retting where jute bundles are submerged into slow running river water and subjected to decomposition of pectin, hemicelluloses, and other mucilaginous substances 2,5 . In this process, pectin is depolymerized by pectinases, primarily comprising four enzymes: Polygalacturonase (PG), Pectin Lyase (PNL), Pectate lyase and Pectin esterase. However, PG 6 , and PNL 7 are primary retting enzymes. In addition, xylanase makes jute fibre softer by selective removal of non-fibrous hemicelluloses without affecting strength of cellulosic fibre. Pectinolytic microorganisms having xylanase activity devoid of cellulase activity is an additional beneficial aspect to improve fibre quality 8 . The quality of fibre is largely determined by the efficiency of retting process 1,2,9,10 and various factors are responsible for proper retting as well as improved fibre quality. Most promising water based microbiological retting process mostly involves bacteria along with various fungi, protozoa, algae and diatoms [10][11][12][13] [14][15][16][17][18] along with large numbers of gram-negative genera such as Erwinia and Pseudomonas 9,19 . At the later stage of retting some anaerobic bacteria from genus Clostridium -Clostridium acetobutylicum, Clostridium stercorarium, Clostridium tertium come to carry on the retting process 20 . As microorganisms are the main pectinolytic agent during retting, affecting the process and end product quality in depth knowledge of microbial community is essential. Moreover, retting water varies from place to place with respect to its physico-chemical, microbial and biochemical properties which affect fibre quality 21,22 . Due to scarcity of water, farmers are compelled to use water bodies repeatedly for retting, leading to poor quality jute fibre production 21,23 . Acute shortage of water and the environmental pollution created from conventional system of retting has demanded for improving the retting process. Aim of this work was to optimize microbial retting protocol that will lower retting period and increase fibre quality. Our strategy involved analysis of pectinolytic retting bacteria with selection of best synergistic effect Identification and phylogenic analysis. A molecular approach based on 16S rRNA gene sequencing was used to identify and distinguish closely related bacterial strains (Supplementary Table 3) and the retrieved sequences were used to construct phylogenetic trees to show relative positions of the isolates at genus level. The 16s rDNA sequence analysis and estimation of phylogenetic relationships (Fig. 2) assigned all 144 strains into two predominant phyla-Firmicutes (most abundant components ~80.55%) and Proteobacteria (~19.45%) which corroborated with the findings of Munshi and Chattoo 2 . The comparative sequence analysis revealed a rich spectrum of bacterial diversity. The total of 144 bacterial isolates belonged to 14 phylogenetically related species-Bacillus aryabhattai (29%), Bacillus subtilis (19.44%), Bacillus cereus (17.36%), Bacillus megaterium (4.86%), Bacillus koreensis (3.47%), Bacillus xiamenensis (2.78%), Staphylococcus arlettae (0.69%), Clostridium aurantibutyricum (2.78%), Aeromonas jandaei (12.5%), Proteus mirabilis (3.47%), Serratia nematodiphila (1.39%), Kosakonia sacchari (0.69%), Kosakonia oryzae (0.69%) and Enterobacter tabaci (0.69%) under 8 genera (Fig. 3). Comparative sequence analysis revealed that 144 isolates belong to phylogenetically related 14 species and the Bacillus spp. was dominant. Many Bacillus sp. are also widely reported to produce enzymes of industrial application in paper industry [28][29][30][31][32][33] and bast fibre degumming 34,35 . The abundance of these species in our study is in accordance with the earlier culture-based studies, which implicate their role in the retting of jute 3,13 . Interestingly, we have identified seven phylogenetically related bacterial species namely Aeromonas jandaei, Proteus mirabilis, Bacillus xiamenensis, Bacillus koreensis, Serratia nematodiphila, Kosakonia oryzae and Enterobacter tabaci as retting bacteria which were not reported in previous study as jute retting bacteria.
Selection of best retting bacterial strains. Out of 144, only 10 bacterial strains were selected from retting niche based on extracellular enzymatic activities for preparing retting consortia ( Comparison of individual and consortial enzyme activity. Strains within various species usually differ in their capacity to ret jute due to varying in enzyme activities. From 10 selected isolates, the highest pectinase activity was noted in Bacillus megaterium (ID-417; 25 mm clear zone, 14.59 U/ml) while lowest was in Kosakonia oryzae (ID-105; 16 mm clear zone, 6.22 U/ml). Aeromonas jandae (ID-191; 23.5 mm clear zone, 6.03 U/ml) and Proteus mirabilis (ID-104; 23.5 mm clear zone, 6.38 U/ml) recorded as the highest xylanase activity while it was lowest in Kosakonia oryzae (ID-105; 15 mm clear zone, 1.63 U/ml) ( Table 1). We observed that the pectinolytic and xylanolytic activities associated with cellulolytic activity. Every pectinolytic microbes found in our study had cellulolytic activity. Brühlmann, and his colleague 36 reported that cellulolytic activities were always found to be associated with pectinolytic and xylanolytic activities.
Based on pectinolytic and xylanolytic activities 10 bacterial isolates were selected for retting consortia. Because, a mixture of microbes secreting different enzymes are more effective for retting of jute plants than a single microbe 37 . Microbial consortia included 10 phylogenetically related species namely, Bacillus megaterium, Bacillus subtilis, Bacillus cereus, Bacillus xiamenensis, Bacillus koreensis, Proteus mirabilis, Enterobacter tabaci, Kosakonia oryzae, Serratia nematodiphila and Aeromonas jandaei. One hundred and sixty seven combinations were evaluated for their enzyme activities (Supplementary Table 4). Finally, three consortia namely C-51, C-67 and C-90 were (having highest pectinolytic and xylanase activities however lower cellulolytic activity) selected as potential for use in large scale jute retting process after screened for antagonism. In most of the cases, all the enzyme activities of the consortia were higher than the individual organisms. For example, consortium C-67 showed higher pectinase (31.5 mm clear zone, 21.4 U/ml) and xylanase (30.5 mm clear zone, 8.56 U/ml) activities (Table 2) corroborating the potentiality of using microbial consortia instead of single microbial strain (Fig. 4).

Effectiveness of bacterial consortia in retting.
Three bacterial consortia, C-51, C-67 and C-90 with an inoculum of 1 × 10 8 CFU/ml concentrations and a 5:1 water-inocula ratio reduced the retting period to 10-11 days from 21days (Table 3). It also made remarkable improvement in jute fibre strength, twisting force and luster over control. The results showed that the fibre strength, twisting force and luster increased when microbial consortia were used for retting compared with positive control. The increment of fibre strength and luster could  www.nature.com/scientificreports www.nature.com/scientificreports/ amount to about 20% and fibre twisting force could amount to 9%. It indicated that retting with microbial consortia could results in the effectively removal of pectinolytic material linking gum component within a short time from the fibre. It also confirmed that the microbial consortia did not damage jute fibre. Tenkanen and his colleague 38 have shown that the residual lignin linking with xylan in birch kraft pulp could be removed by xylanase. Higher fibre strength, twisting force and luster could be achieved by using C-67 consortium compared with C-90 and C-51. The results clearly demonstrated that microbial consortia significantly reduced the retting period as well as improved the fibre quality in respect of strength, twisting force and luster. Among them, C-67   www.nature.com/scientificreports www.nature.com/scientificreports/ consortium gave the best result that reduced the retting time from 18-21days to 10 days with better fibre quality. Thus water-retting process and fibre quality were substantially improved by simultaneously inoculating water tanks with six selected pectinolytic strains. Saha et al. 39 used a microbial consortia for jute retting comprising three strain of Bacillus pumilus which retted jute plants in 13-15 days. But in the current study, bacterial consortia comprising more than one species has been used to reduce retting period from 18-21 days to 10 days. It is also worth mentioning here that the bacterial consortium is capable of improving fibre strength, color and fineness without using any chemical.

conclusion
Jute cultivation in water scarce environment is under threat due to higher water requirements for separating fibre from jute stem through retting process. The present study indicated that selective inoculation with efficient microorganisms could be an alternative method of jute retting to obtain quality fibre in water scarce environment. The consortium C-67 could be adopted after commercial field trial to ret jute in minimum water within short time. Retting sample collection. Five retting liquor samples namely-DRW-1, DRW-2, DRW-3, DRW-4 and DRW-5, were collected at four days interval within 4-20 days of retting from close proximity of submerged mat of jute bundles to get maximum coverage of retting microbial population. Three sub-samples of retting water were collected from evenly spaced parts (upper, middle and lower) of the jute bundle for each sample at a depth of 20 cm from water surface. All the samples were immediately placed on ice for transportation. The three sub-samples were pooled to create a single composite sample and filtered using Cheese cloth (50-100 μm) followed by Mira cloth (25 μm) repeatedly to separate the rough debris. The temperature and pH of the retting water during the retting season was 25-30 °C and 5.04-7.75, respectively.

Methods
Isolation and purification of bacterial strains. The composite samples were diluted up to 10 −5 in peptone water (Peptone 10 g/L, NaCl 5 g/L; pH 7.2 ± 0.2). Then 100 μl of samples from each dilution were spread on Nutrient agar (NA) (Peptone 5 g/L, Yeast extract 2 g/L, Meat extract 1 g/L, NaCl 5 g/L, Agar 15 g/L; pH 7.2 ± 0.2) and incubated at 34 °C for 24 hour in aerobic and anaerobic condition (AnaeroGen ™ AN0035 kit). All the media were collected from Sigma-Aldrich. Triplicate set of plates were used for all the treatments throughout the study. Bacterial colonies were picked up based on different appearance and colony characteristics were determined according to Holtz 40 . Enzyme activity of the isolates. Solid culture extra-cellular enzyme assay. Primary screening of the isolates having pectinase, xylanase and cellulase activities was done by single touch inoculation of each colony onto 0.5% pectin, xylan and Carboxymethyl cellulose (CMC) agar respectively and incubated at 34 °C for 24 hours. Plates were observed for enzyme activity by flooding them with iodine solution (Iodine 1 g and Potassium Iodide 5 g for 330 ml iodine solution) 41 Table 3. Average retting period and quality parameter of jute fiber.
Scientific RepoRtS | (2020) 10:5174 | https://doi.org/10.1038/s41598-020-61898-z www.nature.com/scientificreports www.nature.com/scientificreports/ Quantitative extra-cellular enzyme assay. Quantitative enzyme assay of retting isolates was based on the determination of reducing sugars produced as a result of enzymatic hydrolysis of pectin, xylan and cellulose by dinitrosalicylic acid reagent (DNS) method 43 . For the assay, 5 ml bacterial culture grown in modified MS medium containing 0.3% KH 2 PO 4 , 0.6% Na 2 HPO 4 , 0.2% NH 4 Cl, 0.5% NaCl, 0.01% MgSO 4.7 H 2 O supplemented with 0.5% yeast extract and 0.5% pectin (for pectinase production) or xylan (for xylanase production) or carboxymethyl cellulose (for cellulase production) was centrifuged at 10,000 rpm for 10 min at 4 °C and the clear supernatant was used as crude enzyme. Beechwood xylan 1% and carboxymethyl cellulose (CMC) 1% (Sigma-Aldrich) were prepared in 0.05M Na-citrate buffer of pH 5.3 and pH 4.8 respectively. Whereas Polygalacturonic acid 0.5% was prepared in 0.1M phosphate buffer (pH 7.5) and used as substrates for xylanase, cellulase and pectinase. The reaction mixture contained 900 μl of respective substrate (pectin and xylan) and 100 μl of appropriately diluted enzyme (pectinase, and xylanase), whereas, 100 μl of distilled water was used for enzyme blank. In case of cellulase, 1 ml of substrate (CMC) and 1 ml of appropriately diluted crude enzyme were used and were incubated at 50 °C for 10 min and the reaction was terminated by adding 1 mL of 3,5-dinitrosalicylic acid (DNS) and boiling (92 °C) for 5 min. Finally, the tubes were cooled and optical density (OD) was measured using spectrophotometer (Bio-Rad SmartSpec Plus) at 540 nm. For pectin, xylan and CMC, reducing sugar concentrations were estimated as D-galacturonic acid D-xylose and D-glucose equivalents, using a calibration curve constructed with D-galacturonic acid (Sigma-Aldrich, ≥98.0% purity) D-xylose (Sigma-Aldrich, ≥99% purity) and D-glucose (Sigma-Aldrich, ≥99.5% purity) respectively. The enzyme unit (U) was defined as the amount of enzyme that catalyzes the formation of 1 μmol of reducing sugar per minute under the specified assay conditions.
Isolation of genomic DNA. Genomic DNA was isolated following the method of Sambrook and Russel 44 and treated with RNase A. The quantity and purity of DNA was assessed using a NanoDrop 2000 spectrophotometer (NanoDrop, Thermo Scientific). The integrity of DNA was evaluated by 1% agarose gel electrophoresis. Sequencing of 16S rDNA fragment, assembly and BLAST search. The amplified and purified PCR fragments were sequenced in ABI 3730XL DNA Analyzer (Applied Biosystems, Life Technologies, USA) with the primer 27F (5′-AGAGTTTGATCMTGGCTCAG-3′), 533R (5′-TTACCGCGGCTGCTGGCAC-3′), 981R (5′-GGGTTGCGCTCGTTGCGGG-3′) and 1492R (5′-GGTTACCTTGTTACGACTT-3′). Sequencing reaction was performed by using Big Dye V3.1 sequencing reagents (Applied Biosystems, Life Technologies, USA) following the manufacturer's protocol. The four sequences for each sample were assembled using CAP3 Sequence Assembly Program, to obtain the full 16S rRNA genes. The 16S rDNA sequences of the isolated strains were compared to public databases available in NCBI. Identification to the species level was determined as a 16S rDNA sequence similarity of >99% with that of the prototype strain sequences in the GenBank.
Phylogenetic analysis. The 16S rDNA sequences of isolates were aligned with the MUSCLE and phylogenetic trees were inferred using the neighbor-joining method 45 . The software MEGA, version 6.0, was used to construct trees 46 . Bootstrap analysis (100 replicates) was used to test the topology of the neighbor-joining method.
Extracellular enzymatic assay of bacterial consortia. A total of 167 consortia of different combinations containing 3 to 10 bacterial isolates, were selected to test synergistic effects in extracellular enzyme production. For each treatment, primary inoculum of individual strain was prepared by growing in 20 ml NB at 30 °C for 24 hours which was used to inoculate 99 ml NB in 1:99 ratio after adjustment of Optical Density (OD) at 6-7(±0.4) (A = 600). After attaining mid-log phase (0.4-0.6 OD) of growth, bacterial cultures were mixed equally and OD of mixed culture was adjusted at 6.5-7.0 to inoculate 99 ml NB in 1:99 ratio and incubated for their respective incubation period (Optimization). Enzyme activity was checked according to same procedure as extracellular enzyme assay. The bacterial isolates were further screened for enzyme activity by quantitative assay. To study the pectinase, xylanase and cellulase activities in various consortia, the respective enzyme producing media were simultaneously inoculated with the bacterial strains and the cell free supernatants were used for the assays. The enzyme producing media composition and quantitative enzyme assay procedure were as same as described above in Quantitative extra-cellular enzyme assay section.
Retting efficiency test. Small scale. Artificial plastic retting tanks (Length 150 inch, width 14 inch and depth 7 inch) were used for jute retting trial. Green ribbons were extracted from 120 days aged defoliated jute plant (Corchorus olitorius, variety O-4) with an average height 3.30 m and diameter 23 mm by a ribbon extractor machine (CRIJAF, 2011). Two kg of green ribbon was submerged in 10 L of distilled water at a substrate liquor ratio of 1:5. Three consortia C-51, C-67 and C-90 with 5, 6 and 7 bacterial strains respectively were used as inocula in each treatment. The bacterial inocula were added with water of 10:1 at 1 × 10 8 cells/ml. Plastic tanks were covered with cork sheet and kept at green house to maintain the temperature at 30-32 °C until completion of