<i>Leuconostoc citreum </i>and use thereof in precipitating starch emulsion

Abstract

Provided is a method for precipitating a starch emulsion, the method including: mixing a fermentation broth with the starch emulsion, the fermentation broth including an isolated microorganism, wherein the isolated microorganism is Leuconostoc citreum WSJ-57 deposited under an accession number of CGMCC No. 19201 in the China General Microbiological Culture Collection Center on Dec. 20, 2019.

Claims

1. A method for precipitating a starch emulsion, the method comprising: mixing (i) a fermentation broth containing a culture of Leuconostoc citreum WSJ-57, deposited under accession number CGMCC No. 19201, with (ii) a starch emulsion, to produce a mixture; and performing stand treatment of the mixture sufficient to precipitate the starch emulsion.

2. The method according to claim 1, wherein a concentration of the Leuconostoc citreum WSJ-57 in the fermentation broth ranges from 1?10.sup.9 CFU/mL to 5?10.sup.9 CFU/mL, a starch concentration of the starch emulsion ranges from 10 g/L to 40 g/L, and a volume ratio of the fermentation broth to the starch emulsion ranges from 1:10 to 1:15.

Description

BRIEF DESCRIPTION OF DRAWINGS

(1) The above and/or additional aspects and advantages of the present disclosure will become apparent and easily understandable from the description of embodiments with reference to the following drawings, in which:

(2) FIG. 1 schematically illustrates effect comparison of a control group and a treatment group at a time when precipitating a starch emulsion with Leuconostoc citreum according to an embodiment of the present disclosure for 1 min;

(3) FIG. 2 schematically illustrates effect comparison of a control group and a treatment group at a time when precipitating a starch emulsion with Leuconostoc citreum according to an embodiment of the present disclosure for 3 min;

(4) FIG. 3 schematically illustrates effect comparison of a control group and a treatment group at a time when precipitating a starch emulsion with Leuconostoc citreum according to an embodiment of the present disclosure for 15 min;

(5) FIG. 4 illustrates a phylogenetic tree of gene sequence of SJ-57 strain according to an embodiment of the present disclosure;

(6) FIG. 5 illustrates a schematic diagram of an identification result analysis of BIOLOG automatic micro-analysis system according to an embodiment of the present disclosure; and

(7) FIG. 6 illustrates a colony morphology of SJ-57 strain in a MRS agar medium according to an embodiment of the present disclosure.

DESCRIPTION OF EMBODIMENTS

(8) Solutions of the present disclosure will be explained with examples below. Those skilled in the art will understand that the following examples are only used to illustrate the present disclosure, and should not be regarded as limitations of the scope of the present disclosure. The specific technologies or conditions that are not indicated in the embodiments shall be those described in the literatures in the related field or according to the product manuals. The reagents or instruments without specifying the manufacturers are conventional products that are commercially available.

Example 1

(9) I. Isolating and Purifying Lactobacilli

(10) 1. 10 ml of naturally fermented sour liquor of sweet potato was mixed with 90 ml of sterile physiological saline to prepare gradient diluted sample suspensions, with the gradient concentrations of 10.sup.?1, 10.sup.?2, 10.sup.?3, 10.sup.?4, 10.sup.?5 and 10.sup.?6.

(11) 2. Using a MRS medium as a selective medium, 200 ?l of each gradient diluent was evenly coated on the MRS agar medium, and cultured at 37? C. for 48 h to obtain a single colony.

(12) 3. Plates corresponding to the gradient concentrations of 10.sup.?4, 10.sup.?5 and 10.sup.?6 were selected as screening objects, and for each plate, one single representative pure colony with a different shape was selected, and the obtained single colony was continuously purified twice by mean of zigzag streaking and three-zone streaking. 74 single colonies were purified in total, each of them was picked and put into a MRS broth, and cultured at 37? C. for 48 hours.

(13) 4. The purified bacteria solutions were numbered with SJ-1 to SJ-74; under aseptic conditions, the bacteria solution was mixed with sterilized glycerol with a concentration of 50% in a volume ratio of 1:1 in a frozen storage tube, and a final concentration of the glycerol was 25%, and the mixture was stored in a refrigerator at ?80? C.

(14) 5. The MRS agar medium contained the following components: 10.0 g of peptone, 8.0 g of beef extract powder, 4.0 g of yeast extract powder, 20.0 g of glucose, 2.0 g of dipotassium hydrogen phosphate, 2.0 g of diammonium hydrogen citrate, 5.0 g of sodium acetate, 0.2 g of magnesium sulfate, 0.04 g of manganese sulfate, 14.0 g of agar, 1.0 g of tween 80, with a pH value of 6.5?0.2, and the volume was adjusted to 1 L with water.

(15) 6. The MRS broth culture medium contained the following components: 10.0 g of peptone, 8.0 g of beef extract powder, 4.0 g of yeast extract powder, 20.0 g of glucose, 2.0 g of dipotassium hydrogen phosphate, 2.0 g of diammonium hydrogen citrate, 5.0 g of sodium acetate, 0.2 g of magnesium sulfate, 0.04 g of manganese sulfate, 1.0 g of tween 80, with a pH value of 6.5?0.2, and the volume was adjusted to 1 L with water.

(16) II. Screening Strains for High-Efficient Flocculating and Precipitating Starch

(17) 1. The strains with serial numbers of SJ-1 to SJ-74 were activated, rejuvenated, inoculated and expanded for culture. The specific operation was as follows: dipping the bacteria solution in a glycerol tube with a sterile inoculation ring, culturing it on a MRS agar medium by means of zigzag streaking and three-zone streaking at 37? C. for 48 h, and selecting and culturing a single colony in a MRS broth at 37? C. for 48 h, where the bacteria solution was the seed solution; adsorbing the seed culture solution and inoculating in a 10 ml MRS broth for expanded culture according to a volume ratio of 1%, so as to obtain a pure bacterial fermentation solution; culturing each strain to a stable stage, and controlling the concentration of the bacteria solution to be 1.2?10.sup.9 CFU/ml.

(18) 2. Using flocculation rate and starch yield as screening indexes, 2 ml of pure bacteria solution was added into 25 ml of sweet potato starch emulsion (25 g/L), and then it was left to settle for 20 min; the flocculation rate and starch yield of the starch emulsion under the effect of each strain were calculated, and the strain with the highest activity in terms of starch flocculation and precipitation was screened.

(19) 3. The flocculation rate of the starch emulsion was determined as follows. two parts of 25 ml of starch emulsion (25 g/L) were prepared with distilled water and sweet potato starch, one of the two parts for control and the other for treatment. The bacteria solution was shaken evenly and divided into two parts; 2 ml of one part of the bacteria solution was added into the starch emulsion for treatment, shaken up down for 1 min and stood for 20 min; the supernatant was taken at a level of 1 cm below the liquid surface and the absorbance thereof was measured on a visible spectrophotometer, at a wavelength of 550 nm, which served as the treated sample and designated as A.sub.2. The other part of bacteria solution was inactivated first, then centrifuged and discarded the supernatant to obtain the bacteria, and then added with the same volume of fresh MRS broth was prepared as a control bacteria solution; 2 ml of the control bacteria solution was added to the control starch emulsion; the remaining steps were the same as those for the treated sample, the measured absorbance was recorded as A.sub.1.

(20) The flocculation rate was calculated with the following equation:
FR=(A.sub.1?A.sub.2)/A.sub.1?100%,

(21) where A.sub.1 represents OD.sub.550 of the control supernatant, and A.sub.2 represents OD.sub.550 of the treated supernatant.

(22) 4. The starch yield was determined as follows. 25 ml of starch emulsion (25 g/L) was prepared with distilled water and sweet potato starch, and 2 ml of a fermentation broth was added into the starch emulsion and shaken up and down for 1 min and then stood for 20 min for precipitation; then, the supernatant of the starch emulsion was discarded, the precipitated starch was placed into an oven and dried for 3 h to a constant weight, taken out and cooled to room temperature in a desiccator, weighed, and then placed back into the oven and dried for 0.5 h to a constant weight, cooled and weighed until the difference between the masses before and after the operation was smaller than 0.002 g. The calculation formula was as follows:
Starch yield=mass of precipitated starch (dry basis)/mass of starch in starch emulsion (dry basis)?100%

(23) 5. During the screening process, 7 strains were found to have flocculation and sedimentation effect on the starch emulsion. According to the results in Table 1, the SJ-57 bacteria solution has the highest flocculation rate and starch yield. FIG. 1 to FIG. 3 illustrate the situations of the starch emulsion added with the SJ-57 bacteria solution and the starch emulsion added with the control bacteria solution at times when precipitating for 1 min, 3 min, and 15 min, respectively. It can also be seen from the figures that starch precipitated at the bottom of the starch emulsion added with the SJ-57 bacteria solution is obviously more than that of the control sample.

(24) TABLE-US-00001 TABLE 1 Flocculation rate and starch yield of 7 strains with high flocculation activity isolated from sweet potato acidic steeping liquor Strain No. SJ-5 SJ-14 SJ-36 SJ-45 SJ-46 SJ-48 SJ-57 Flocculation 15.18 ? 3.45 28.74 ? 5.69 27.36 ? 2.78 31.52 ? 9.98 47.78 ? 2.48 33.23 ? 0.06 55.56 ? 2.96 rate % Starch 71.45 ? 0.02 75.01 ? 1.13 74.42 ? 0.15 75.08 ? 0.77 80.07 ? 0.02 77.66 ? 0.66 84.57 ? 0.07 yield %
III. Identification of the SJ-57 Strain

(25) 1. The molecular identification of the SJ-57 was carried out by using the genomic DNA of the SJ-57 as a template to carry out PCR amplification with a universal primer 16S rRNA of bacterial gene. Specific sequencing was performed as follows.

(26) (1) Extraction of bacterial genomic DNA: a bacterial genomic DNA extraction kit was used.

(27) (2) PCR amplification: the universal primer 16S rRNA of bacterial gene was used: 27F: AGAGTTTGATCCTGGCTCAG (SEQ ID NO: 1); 1492R: GGCTACCTTGTTACGACTT (SEQ ID NO: 2). The reaction procedure was as below: pre-denaturation at 95? C. for 10 min, denaturation at 94? C. for 30 seconds, annealing at 55? C. for 30 seconds, extension at 72? C. for 1.5 min, repeated for 30 cycles; extension at 72? C. for 10 min and preserved at 4? C.

(28) (3) Gel electrophoresis: 1% agarose electrophoresis was used, and the electrophoresis was observed after treating at 150 V and 100 mA for 20 min.

(29) (4) Purification and recovery: the target band was cut, and the recovered product was sequenced.

(30) 2. BLAST search of 16S rRNA gene sequence was performed in the NCBI nucleic acid database, and compared with the existing sequences in the database in terms of homology. The results of sample sequencing and splicing were as follows:

(31) TABLE-US-00002 (SEQIDNO:3) ATCTGACTTAGACGGCTCCTCCCGAAGGTTAGGCCACCGGCTTTGGGCATTACAAACTCC 60 CATGGTGTGACGGGCGGTGTGTACAAGACCCGGGAACGTATTCACCGCGGCGTGCTGATC 120 CGCGATTACTAGCGATTCCGACTTCGTGCAGTCGAGTTGCAGACTGCAGTCCGAACTGAG 180 ACGTACTTTAAGAGATTAGCTCACCTTCGCAGGTTGGCAACTCGTTGTATACGCCATTGT 240 AGCACGTGTGTAGCCCAGGTCATAAGGGGCATGATGATCTGACGTCGTCCCCGCCTTCCT 300 CCGGTTTGTCACCGGCAGTCTCGCTAGAGTGCCCAACTGAATGCTGGCAACTAACAATAA 360 GGGTTGCGCTCGTTGCGGGACTTAACCCAACATCTCACGACACGAGCTGACGACGACCAT 420 GCACCACCTGTCACTTTGTCTCCGAAGAGAACACTTCTATCTCTAAAAGCTTCAAAGGAT 480 GTCAAGACCTGGTAAGGTTCTTCGCGTTGCTTCGAATTAAACCACATGCTCCACCGCTTG 540 TGCGGGTCCCCGTCAATTCCTTTGAGTTTCAACCTTGCGGTCGTACTCCCCAGGCGGAAT 600 ACTTAATGCGTTAGCTTCGGCACTAAGAGGCGGAAACCTCCTAACACCTAGTATTCATCG 660 TTTACGGTGTGGACTACCAGGGTATCTAATCCTGTTTGCTACCCACACTTTCGAGCCTCA 720 ACGTCAGTTGTTGTCCAGTAAGCCGCCTTCGCCACTGGTGTTCTTCCATATATCTACGCA 780 TTCCACCGCTACACATGGAGTTCCACTTACCTCTACAACACTCAAGTTAACCAGTTTCCA 840 ATGCCATTCCGGAGTTGAGCTCCGGGCTTTCACATCAGACTTAATCAACCGTCTGCGCTC 900 GCTTTACGCCCAATAAATCCGGATAACGCTCGGGACATACGTATTACCGCGGCTGCTGGC 960 ACGTATTTAGCCGTCCCTTTCTGGTATGGTACCGTCAAACTAAAATCATTCCCTATTTTA 1020 GCATTTCTTCCCATACAACAGTGCTTTACGACCCGAAAGCCTTCATCACACACGCGGCGT 1080 TGCTCCATCAGGCTTGCGCCCATTGTGGAAGATTCCCTACTGCAGCCTCCCGTAGGAGTT 1140 TGGGCCGTGTCTCAGTCCCAATGTGGCCGATCAGTCTCTCAACTCGGCTATGCATCATCG 1200 TCTTGGTAAGCCTTTACCCCACCAACTAACTAATGCACCGCGGATCCATCTCTAGGTGAC 1260 GCCGTAGCGCCTTTTAACTTGATATCATGCGATACTAAGTTTTATTCGGTATTAGCATCT 1320 GTTTCCAAATGTTATCCCCAGCCTTGAGGCAGGTTATCCACGTGTTACTCACCCGTTCGC 1380 CACTCGCTTGAAAGGTGCAAGCACCTCTCGCTGCGCGTCGACTGCATGTATAGCCCCCCC 1440 CC. 1442

(32) The results of homology analysis indicate that the sequence has high homology with each species of Leuconostoc citreum and the homology can be more than 99%.

(33) At the same time, Applicant compared and analyzed the 16S rRNA gene sequences of other strains in Table 1, and identified SJ-5 as Weissella confusa, SJ-14 as Leuconostoc mesenteroides, and SJ-36 as Leuconostoc mesenteroides, SJ-45 as Leuconostoc mesenteroides, SJ-46 as Leuconostoc holzapfelii, and SJ-48 as Leuconostoc mesenteroides.

(34) 3. 16S rRNA gene sequences of related strains were selected from GenBank, Clustal W multiple alignment was carried out by MEGA 7 software, phylogenetic tree was constructed by the Neighbour-joining method, and bootstrap analysis was carried out, with 1000 times of repetitions. The results are illustrated in FIG. 4. It can be seen from the phylogenetic tree that SJ-57 belongs to the same ethnic group as two strains of Leuconostoc citreum, with homology up to 97%.

(35) 4. The SJ-57 strain was identified by a BIOLOG automatic micro-analysis system. The results are illustrated in FIG. 5. Through the identification with such a system, the similarity between SJ-57 and Leuconostoc citreum can be 87.3%. According to the above identification results, the SJ-57 strain was finally identified as one strain of Leuconostoc citreum, named as Leuconostoc citreum WSJ-57. FIG. 6 illustrates a colony morphology of this strain in MRS agar medium.

(36) In the present disclosure, the expressions one embodiment, some embodiments, examples, specific examples, some examples, etc. mean that the specific features, structures, materials, or characteristics described in conjunction with the embodiment or example are included in at least one embodiment or example of the present disclosure. In this specification, the above terms do not necessarily refer to the same embodiment or example. Moreover, the specifically described features, structures, materials or characteristics can be combined in any one or more embodiments or examples in a suitable manner. In addition, those skilled in the art can combine the different embodiments or examples and the features of the different embodiments or examples described in this specification without contradicting each other.

(37) Although the embodiments of the present disclosure have been shown and described above, it can be understood that the above-mentioned embodiments are exemplary and should not be construed as limitations of the present disclosure. Those skilled in the art can make changes, modifications, replacements and modifications to the above-mentioned embodiments without departing from the scope of the present disclosure.