Method for regulating expression of protein of interest in bacillus subtilis
10975377 · 2021-04-13
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Inventors
Cpc classification
International classification
Abstract
The present disclosure relates to a method for regulating expression of protein of interest in Bacillus subtilis, and belongs to the technical field of genetic engineering. The method comprises: using Bacillus subtilis as an expression host, adding the N-terminal nucleotide sequence coding the first 15 amino acids of the endogenous protein before the coding gene of the protein of interest or modifying the original N-terminal nucleotide sequence coding the first 15 amino acids, and performing free expression in plasmid, thereby regulating expression of the protein of interest in Bacillus subtilis, and even regulating the expression difference in different growth phases and the expression level.
Claims
1. A method for regulating expression of a protein in Bacillus subtilis, comprising: modifying a gene encoding the protein by adding upstream thereto nucleotide sequence SEQ ID NO:18 to obtain a modified gene encoding a recombinant protein, transferring the modified gene encoding the recombinant protein into an expression vector, and transfecting Bacillus subtilis with the expression vector for expression of the recombinant protein, and inducing expression of the expression vector.
2. The method according to claim 1, wherein the Bacillus subtilis strain is any one or more of: Bacillus subtilis 168, Bacillus subtilis WB400, Bacillus subtilis WB600, and Bacillus subtilis WB800.
3. The method according to claim 1, wherein the expression vector comprises pP43NMK.
4. The method according to claim 1, wherein the protein comprises an enzyme.
5. A vector comprising the modified gene encoding the recombinant protein of claim 1.
Description
BRIEF DESCRIPTION OF FIGURES
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DETAILED DESCRIPTION
(12) (1) Recombinant Bacillus subtilis seed culture and fermentation
(13) Medium (g/L): tryptone 10, yeast powder 5, NaCl 10.
(14) Culture conditions: transferring seeds cultured at 37° C., 200 rpm for 10 h to the fermentation medium according to an inoculum size of 10% (v/v), and culturing the seeds at 37° C., 200 rpm for 20 h.
(15) (2) Method for determining the expression level of green fluorescent protein
(16) Adding 200 μL of diluted fermentation broth to each well in a 96-well plate, and using a Cytation 3 cell imaging microplate reader (Berton Instruments, Inc., USA), specifically, excitation wavelength: 488 nm, emission wavelength: 523 nm, and gain: 60.
Example 1
Effects of Addition of Nucleotide Sequences as Shown in SEQ ID NO.1-SEQ ID NO.109 to N-Terminal on Expression of Green Fluorescent Protein in Engineering Bacteria
(17) 1. Construction of Recombinant Plasmid
(18) The composition of recombinant plasmid is that the nucleotide sequence to be added and the green fluorescent protein (GFP) gene are sequentially inserted after the P43 promoter of Pp43NMK plasmid.
(19) To introduce the nucleotide sequence to be added after the P43 promoter, primers rh_CspD-0.75k_p43NMK-GFP_F: 5′-TGGTTCAACGAAAAAGGATTCATGAGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCA-3′ (i e SEQ ID NO. 152), and rh_CspD-0.75k_p43NMK-GFP_R: 5′-TACGCCAAGCTTTCATCACTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAG-3′ (i e SEQ ID NO.153) were designed, Escherichia coli containing the green fluorescent protein (GFP, GenBank: AF324408.1) gene was used as a template, and a green fluorescent protein fragment was obtained by colony PCR.
(20) Primers fx_CspD-6.7k_p43NMK-GFP_F: 5′-AGTGATGAAAGCTTGGCGTAATCATGGTCATAGCTGTTT-3′ (i e SEQ ID NO.154), and fx_CspD-6.7k_p43NMK-GFP_R: 5′-CCTTTTTCGTTGTTGAACCATTTTACTTTACCGTTTTGCATGTGTACATTCCTCTCTTACCTATAATGGTACCGCTATCACTT-3′ (i e SEQ ID NO.155) were designed. Plasmid pP43NMK was used as a template and a plasmid fragment was obtained by reverse amplification by PCR. Finally, the recombinant plasmid was constructed by Gibson Assembly Clonging Kit (New England Biolabs), and it was verified that the construction of the recombinant pP43NMK-TufAN-GFP plasmid is successful by sequencing.
(21) 2. Construction of Recombinant pP43NMK-CspDN-GFP Plasmid Bacillus Subtilis
(22) The constructed pP43NMK-CspDN-GFP plasmid was transformed into a wild type strain of Bacillus subtilis 168. Primers yz_zong-p43NMK_F: 5′-TTCTTGCTGAGTCTGGCTTTCG-3′ (i e SEQ ID NO.156) and yz_zong-p43NMK_R: 5′-CGGCTCGTATGTTGTGTGGAAT-3′ (i e SEQ ID NO.157) was used to select transformants for colony PCR, and it was verified that the construction of the recombinant Bacillus subtilis is successful when a 1.8 kb band appeared.
(23) 3. Expression of Green Fluorescent Protein in Engineering Bacteria After Addition of Nucleotide Sequences as Shown in SEQ ID NO.1-SEQ ID NO.109 to N-Terminal
(24) Seeds of the successfully constructed recombinant Bacillus subtilis cultured at 37° C., 750 rpm in a 700 μL LB medium and in a 96-well plate for 9 h were transferred to a 190 μL LB medium according to an inoculum size of 5% (v/v), and cultured at 37° C., 750 rpm for 4 h and 20 h. Under the same conditions, if only expressed by pP43NMK, with no regulatory N-terminal nucleotide sequence added, the average fluorescent intensity in the final fermentation broth was about 5159 measured after 4 h, and about 48181 after 20 h. While after the N-terminal sequence of GLNA protein was added, the average fluorescent intensity was 20912.3 measured after 4 h, and the average fluorescent intensity was 105441.4 after 20 h, which were respectively 4 times and 2 times of that of the control.
(25) The effects of addition of the nucleotide sequences as shown in SEQ ID NO.1-SEQ ID NO.109 to the N-terminal on expression of green fluorescent protein in engineering bacteria is summarized as follows:
(26) (1) The effects of regulating protein expression: the expression level of protein is characterized by fluorescent intensity. According to the fluorescent intensity determination method described herein, the range of expression level of protein regulated by the N-terminal sequence element spans four orders of magnitude. The expression level of protein can be increased by about 7 times compared to the control. In the nucleotide sequence which increases the protein expression level, when the sequence added to the N-terminal is the N-terminal nucleotide sequence (i.e. SEQ ID NO.18) coding the first 15 amino acids of YdbP protein, and the fermentation time is 4 h, the average fluorescent intensity is increased from about 5159 to 35,837, and when the fermentation time is 20 h, the fluorescent intensity is increased from about 48181 to 138986, which are respectively increased to 6.95 times and 2.88 times of that of the control. In the N-terminal nucleotide sequence which decreases the protein expression level, when the sequence added to the N-terminal is the N-terminal nucleotide sequence (i.e. SEQ ID NO.107) coding the first 15 amino acids of RspD protein, and the fermentation time is 4 h, the average fluorescent intensity is decreased from about 5159 to 55, and when the fermentation time is 20 h, the fluorescent intensity is decreased from about 48181 to 1125, which are respectively decreased to 0.011 time and 0.023 time of that of the control. The regulation effects of addition of 109 different specific nucleotide sequences on the expression of green fluorescent protein are shown in Tables 1-4.
(27) (2) The effects of regulating the difference in protein expression in different growth phases: the expression level of protein is characterized by fluorescent intensity. According to the fluorescent intensity determination method described herein, the N-terminal sequence element can regulate differential expression of the protein of interest in different growth phases of Bacillus subtilis, and are divided into growth-coupled pattern, growth-delayed pattern, consistent expression pattern and inhibitory pattern. In the growth-coupled pattern, using the N-terminal sequence of Hbs protein (i.e. SEQ ID NO.1) as an example, the protein expression is mainly concentrated within 10 h, i.e., before the end of the growth logarithm (
(28) TABLE-US-00001 TABLE 1 Effects of growth-coupled pattern N-terminal nucleotide sequence on protein expression Fermentation time 4 h 20 h Average Average N-terminal fluorescent fluorescent sequence number intensity Error Gain intensity Error Gain SEQ ID NO. 1 29414.20 346.01 5.70 75686.25 1841.23 1.57 SEQ ID NO. 2 19751.75 330.34 3.83 38773.67 856.29 0.80 SEQ ID NO. 3 16854.80 402.15 3.27 38603.00 1873.35 0.80 SEQ ID NO. 4 14383.60 439.30 2.79 33570.60 681.03 0.70 SEQ ID NO. 5 13959.00 73.27 2.71 34834.00 1057.41 0.72 SEQ ID NO. 6 10603.40 226.51 2.06 19196.25 825.25 0.40 SEQ ID NO. 7 10244.80 152.32 1.99 13512.96 415.43 0.28 SEQ ID NO. 8 10085.00 278.36 1.95 29682.67 678.99 0.62 SEQ ID NO. 9 7655.60 390.59 1.48 14547.20 817.08 0.30 SEQ ID NO. 10 7153.20 136.10 1.39 17905.20 1407.45 0.37 SEQ ID NO. 11 7045.50 589.50 1.37 17436.50 55.50 0.36 SEQ ID NO. 12 6954.40 324.35 1.35 19980.80 2406.37 0.41 SEQ ID NO. 13 5659.33 54.06 1.10 17053.67 1177.22 0.35 SEQ ID NO. 14 4909.60 207.80 0.95 5833.20 428.00 0.12 SEQ ID NO. 15 3559.20 30.79 0.69 6232.00 436.98 0.13
(29) TABLE-US-00002 TABLE 2 Effects of growth-delayed pattern N-terminal nucleotide sequence on protein expression Fermentation time 4 h 20 h Average Average N-terminal fluorescent fluorescent sequence number intensity Error Gain intensity Error Gain SEQ ID NO. 16 6531.00 310.18 1.27 66030.47 804.18 1.37 SEQ ID NO. 17 5384.40 66.74 1.04 59055.40 773.50 1.23
(30) TABLE-US-00003 TABLE 3 Effects of persistent expression pattern N-terminal nucleotide sequence on protein expression Fermentation time 4 h 20 h Average Average N-terminal fluorescent fluorescent sequence number intensity Error Gain intensity Error Gain SEQ ID NO. 18 35836.80 337.00 6.95 138985.86 353.10 2.88 SEQ ID NO. 19 23509.80 173.96 4.56 75249.75 1820.29 1.56 SEQ ID NO. 20 23045.80 324.31 4.47 89647.50 511.50 1.86 SEQ ID NO. 21 22951.60 348.70 4.45 83260.30 871.40 1.73 SEQ ID NO. 22 21945.80 142.44 4.25 67284.80 692.00 1.40 SEQ ID NO. 23 21802.13 289.37 4.23 114839.71 878.13 2.38 SEQ ID NO. 24 20912.30 769.39 4.05 105441.36 3150.72 2.19 SEQ ID NO. 25 20797.80 481.64 4.03 68119.80 181.00 1.41 SEQ ID NO. 26 20088.00 331.23 3.89 96630.34 3163.70 2.01 SEQ ID NO. 27 17889.05 318.81 3.47 82486.00 1029.00 1.71 SEQ ID NO. 28 17256.20 399.50 3.34 111246.91 1466.33 2.31 SEQ ID NO. 29 15324.89 526.42 2.97 82620.80 2808.92 1.71 SEQ ID NO. 30 14258.40 335.07 2.76 84556.40 1833.33 1.75 SEQ ID NO. 31 13612.60 147.36 2.64 54321.00 1047.92 1.13 SEQ ID NO. 32 13603.20 253.72 2.64 47903.20 3804.04 0.99 SEQ ID NO. 33 13125.60 389.66 2.54 48212.50 83.50 1.00 SEQ ID NO. 34 12150.20 376.38 2.36 56608.67 846.96 1.17 SEQ ID NO. 35 11568.20 136.24 2.24 57555.50 1533.43 1.19 SEQ ID NO. 36 10566.00 228.69 2.05 46124.75 1728.34 0.96 SEQ ID NO. 37 10072.44 333.26 1.95 31078.27 515.74 0.65 SEQ ID NO. 38 9963.20 104.03 1.93 48847.30 581.14 1.01 SEQ ID NO. 39 9869.00 163.03 1.91 45881.00 710.48 0.95 SEQ ID NO. 40 9797.00 251.75 1.90 53319.00 239.00 1.11 SEQ ID NO. 41 9162.82 108.49 1.78 18175.10 1096.50 0.38 SEQ ID NO. 42 9024.38 111.53 1.75 22141.35 630.73 0.46 SEQ ID NO. 43 8809.52 82.33 1.71 15728.10 748.38 0.33 SEQ ID NO. 44 7788.86 44.34 1.51 22172.27 639.97 0.46 SEQ ID NO. 45 7146.97 497.00 1.39 15131.30 819.34 0.31 SEQ ID NO. 46 6699.40 107.45 1.30 18106.50 689.82 0.38 SEQ ID NO. 47 6474.20 78.58 1.25 26126.00 2018.29 0.54 SEQ ID NO. 48 6432.00 358.36 1.25 23656.75 876.07 0.49 SEQ ID NO. 49 6360.55 176.32 1.23 22855.40 1123.12 0.47 SEQ ID NO. 50 5986.60 143.00 1.16 16732.25 388.09 0.35 SEQ ID NO. 51 5914.20 215.96 1.15 19270.13 269.82 0.40 SEQ ID NO. 52 5615.46 151.52 1.09 28803.20 1405.52 0.60 SEQ ID NO. 53 5391.60 177.68 1.05 29367.00 69.00 0.61 SEQ ID NO. 54 5186.80 164.15 1.01 21933.47 1350.77 0.46 SEQ ID NO. 55 4905.60 253.58 0.95 28629.67 522.02 0.59 SEQ ID NO. 56 4836.97 69.30 0.94 11572.60 703.06 0.24 SEQ ID NO. 57 4690.37 183.49 0.91 13302.60 582.46 0.28 SEQ ID NO. 58 4485.46 252.50 0.87 11861.60 501.86 0.25 SEQ ID NO. 59 4447.20 295.91 0.86 16007.50 451.77 0.33 SEQ ID NO. 60 4438.10 167.55 0.86 8401.60 564.91 0.17 SEQ ID NO. 61 3894.00 103.93 0.75 20521.60 886.87 0.43 SEQ ID NO. 62 3659.42 48.73 0.71 7100.00 414.57 0.15 SEQ ID NO. 63 3364.40 91.35 0.65 8628.20 643.51 0.18 SEQ ID NO. 64 3259.99 13.18 0.63 14573.35 662.25 0.30 SEQ ID NO. 65 3026.00 101.30 0.59 12411.20 518.47 0.26 SEQ ID NO. 66 2825.40 66.11 0.55 4809.20 201.14 0.10 SEQ ID NO. 67 2792.20 31.94 0.54 13054.20 586.12 0.27 SEQ ID NO. 68 2791.20 100.59 0.54 8027.40 475.02 0.17 SEQ ID NO. 69 2722.00 42.99 0.53 7114.60 526.61 0.15 SEQ ID NO. 70 2621.60 82.95 0.51 8051.20 791.16 0.17 SEQ ID NO. 71 2602.40 84.76 0.50 3911.20 350.91 0.08 SEQ ID NO. 72 2503.07 19.12 0.49 5894.27 131.82 0.12 SEQ ID NO. 73 2422.00 111.74 0.47 8996.25 164.41 0.19 SEQ ID NO. 74 2339.99 101.48 0.45 5425.40 448.66 0.11 SEQ ID NO. 75 2323.00 65.08 0.45 8277.40 548.11 0.17 SEQ ID NO. 76 2260.00 209.63 0.44 9925.33 414.96 0.21 SEQ ID NO. 77 2128.00 86.23 0.41 7977.80 238.28 0.17 SEQ ID NO. 78 2015.27 98.89 0.39 4215.20 301.67 0.09 SEQ ID NO. 79 1943.20 150.95 0.38 6817.75 221.47 0.14 SEQ ID NO. 80 1909.00 25.65 0.37 8892.40 376.89 0.18 SEQ ID NO. 81 1852.80 23.86 0.36 7207.60 276.46 0.15 SEQ ID NO. 82 1823.40 89.14 0.35 6360.80 496.35 0.13 SEQ ID NO. 83 1749.40 75.94 0.34 6651.75 282.99 0.14 SEQ ID NO. 84 1691.20 81.25 0.33 3745.25 318.03 0.08 SEQ ID NO. 85 1389.00 65.97 0.27 9258.20 104.10 0.19 SEQ ID NO. 86 1188.00 56.33 0.23 8448.04 101.37 0.18 SEQ ID NO. 87 1085.80 38.30 0.21 4214.40 236.05 0.09 SEQ ID NO. 88 1056.40 24.02 0.20 3152.40 18.25 0.07 SEQ ID NO. 89 878.67 73.91 0.17 2963.80 111.71 0.06 SEQ ID NO. 90 400.55 43.38 0.08 3622.40 295.72 0.08 SEQ ID NO. 91 31097.37 389.49 6.03 7334.80 129.16 2.75 SEQ ID NO. 92 20571.67 335.67 3.99 5286.20 140.43 1.98 SEQ ID NO. 93 29874.33 505.80 5.79 7127.00 69.77 2.67 SEQ ID NO. 94 15592.69 463.03 3.02 3875.40 31.53 1.45 SEQ ID NO. 95 26928.35 666.94 5.22 6938.80 69.44 2.60 SEQ ID NO. 96 30069.00 310.65 5.83 8549.20 130.19 3.20 SEQ ID NO. 97 16593.99 299.46 3.22 2699.20 53.34 1.01 SEQ ID NO. 98 34317.64 598.92 6.65 8460.80 224.50 3.17 SEQ ID NO. 99 33091.00 969.69 6.41 9134.60 272.43 3.42 SEQ ID NO. 100 31810.76 1080.67 6.17 5558.40 250.04 2.08 SEQ ID NO. 101 26750.70 915.80 5.19 6420.60 168.96 2.40 SEQ ID NO. 102 33829.93 290.91 6.56 8101.20 229.42 3.03
(31) TABLE-US-00004 TABLE 4 Effects of inhibitory pattern N-terminal nucleotide sequences on protein expression Fermentation time 4 h 20 h Average Average N-terminal fluorescent fluorescent sequence number intensity Error Gain intensity Error Gain SEQ ID NO. 103 415.60 30.37 0.08 1228.20 56.40 0.03 SEQ ID NO. 104 281.80 31.58 0.05 990.20 49.25 0.02 SEQ ID NO. 105 167.16 17.95 0.03 671.00 72.92 0.01 SEQ ID NO. 106 106.97 22.57 0.02 1203.60 173.20 0.02 SEQ ID NO. 107 55.27 8.07 0.01 1125.00 87.28 0.02 SEQ ID NO. 108 48.10 13.22 0.01 0.00 13.54 0.00 SEQ ID NO. 109 0.00 14.14 0.00 178.60 71.78 0.00
Example 2
Effects of Modification of N-Terminal Sequence on the Expression of Green Fluorescent Protein in Engineering Bacteria
(32) 1. Construction of Recombinant Plasmid
(33) The composition of the recombinant plasmid is that the N-terminal sequence element and the green fluorescent protein (GFP) gene are sequentially inserted after the P43 promoter of Pp43NMK plasmid. To introduce the N-terminal sequence element after the P43 promoter, primers rh_sigw-0.75k_p43NMK-GFP_F: 5′-GATGATTAAAAAAAACATTAAACAAAACAAAAAAAACATGAGTAAAGGAGAAGAACTTTTCACTGGAG-3′ (i.e. SEQ ID NO.158), and rh_sigw-0.75k_p43NMK-GFP_R: 5′-AGTGATGAAAGCTTGGCGTAATCATGGTCATAGCTGTTT-3′ (i.e. SEQ ID NO.152) were designed. Escherichia coli containing the green fluorescent protein (GFP, GenBank: AF324408.1) gene was used as a template, and a green fluorescent protein fragment was obtained by colony PCR. Primers fx_sigw-6.7k_p43NMK-GFP_F: 5′-TTACACATGGCATGGATGAACTATACAAATAGTGATGAAAGCTTGGCGTAATCATGGTCATAGCTG-3′ (i.e. SEQ ID NO.159), and fx_sigw-6.7k_p43NMK-GFP_R: 5′-TGTTTAATGTTTTTTTTAATCATCATTTCCATGTGTACATTCCTCTCTTACCTATAATGGTACC-3′ (i.e. SEQ ID NO.160) were designed.
(34) Plasmid pP43NMK was used as a template and a plasmid fragment was obtained by reverse amplification by PCR. Finally, the recombinant plasmid was constructed by Gibson Assembly Clonging Kit (New England Biolabs), and it was verified that the construction of the recombinant pP43NMK-TufAN-GFP plasmid was successful by sequencing.
(35) 2. Construction of Recombinant pP43NMK-sigw-GFP Plasmid Bacillus Subtilis
(36) The constructed pP43NMK-GLNA-GFP plasmid was transformed into a wild type strain of Bacillus subtilis 168. Primers yz_zong-p43NMK_F: 5′-TTCTTGCTGAGTCTGGCTTTCG-3′ (i.e. SEQ ID NO.156) and yz_zong-p43NMK_R: 5′-CGGCTCGTATGTTGTGTGGAAT-3′ (i.e. SEQ ID NO.157) were used to select transformants for colony PCR, and it was verified that the construction of the recombinant Bacillus subtilis is successful when a 1.8 kb band appeared.
(37) 3. Expression of Green Fluorescent Protein in Engineering Bacteria After Addition of Artificially Designed N-Terminal Sequence Element
(38) A recombinant Bacillus subtilis seed solution cultured at 37° C., 750 rpm in a 700 μL LB medium and in a 96-well deep-well plate for 9 h was transferred to a 190 μL LB medium according to an inoculum size of 5% (v/v), and the seed solution was cultured at 37° C., 750 rpm for 4 h to obtain a recombinant Bacillus subtilis culture solution sample. Under the same conditions, after the recombinant Bacillus subtilis with addition of the original N-terminal sequence element (i e SEQ ID NO.139) was fermented for 4 h, the average fluorescent intensity measured in the fermentation broth was about 22716. While after the artificially designed N-terminal sequence element (i e SEQ ID NO.111) was added, the average fluorescent intensity of the culture solution was 34819 after the recombinant Bacillus subtilis is cultured for 4 hours.
(39) The effects of 14 different original N-terminal sequence elements on the expression level of green fluorescent protein after artificial modification is shown in Table 5.
(40) TABLE-US-00005 TABLE 5 Effects of 21 artificially designed N-terminal sequence elements on protein expression Decrease of Original N- Relative Increase of Relative expression Relative terminal fluorescent expression level fluorescent level by fluorescent sequence intensity by modification intensity Gain modification intensity Gain SEQ ID NO. 138 32608 SEQ ID NO. 110 42986 1.32 SEQ ID NO. 124 5310 0.16 SEQ ID NO. 139 22716 SEQ ID NO. 111 34819 1.53 SEQ ID NO. 125 903 0.04 SEQ ID NO. 140 22321 SEQ ID NO. 112 40543 1.82 SEQ ID NO. 126 433 0.02 SEQ ID NO. 141 22224 SEQ ID NO. 113 37861 1.70 SEQ ID NO. 127 1314 0.06 SEQ ID NO. 142 20756 SEQ ID NO. 114 27496 1.32 SEQ ID NO. 128 1727 0.08 SEQ ID NO. 143 16895 SEQ ID NO. 115 32362 1.92 SEQ ID NO. 129 650 0.04 SEQ ID NO. 144 20034 SEQ ID NO. 116 37069 1.85 SEQ ID NO. 130 5518 0.28 SEQ ID NO. 145 416 SEQ ID NO. 117 5171 12.44 SEQ ID NO. 146 282 SEQ ID NO. 118 7712 27.37 SEQ ID NO. 147 167 SEQ ID NO. 119 7270 43.49 SEQ ID NO. 148 107 SEQ ID NO. 120 10280 96.11 SEQ ID NO. 149 55 SEQ ID NO. 121 21948 397.10 SEQ ID NO. 150 48 SEQ ID NO. 122 8123 168.86 SEQ ID NO. 151 0 SEQ ID NO. 123 7074 /
Example 3
Effects 2 of Addition of Artificially Designed N-Terminal Sequence Elements on Expression of Green Fluorescent Protein in Engineering Bacteria
(41) 1. Construction of Recombinant Plasmid
(42) The composition of the recombinant plasmid is that the N-terminal sequence element and the green fluorescent protein (GFP) gene are sequentially inserted after the P43 promoter of Pp43NMK plasmid. To introduce the N-terminal sequence element after the P43 promoter, primers rh_NO132-0.75k_p43NMK-GFP_F: 5′-CTGCAGTTACCTGCTAAACCAGATATGAGTAAAGGAGAAGAACTTTTCACTGGAG-3′ (i.e. SEQ ID NO.161), and rh_NO132-0.75k_p43NMK-GFP_R: 5′-CGATATCTTCTCTAGTGTACTTTGCCATGTGTACATTCCTCTCTTACCTATAATGGTACCGCTATCACTT-3′ (i.e. SEQ ID NO.162) were designed, Escherichia coli containing the green fluorescent protein (GFP, GenBank: AF324408.1) gene was used as a template, and a green fluorescent protein fragment was obtained by colony PCR. Primers fx_NO132-6.7k_p43NMK-GFP_F: 5′-AGTGATGAAAGCTTGGCGTAATCATGGTCATAGCTGTTT-3′ (i.e. SEQ ID NO.152), and fx_NO132-6.7k_p43NMK-GFP_R: 5′-GGTTTAGCAGGTAACTGCAGCATCAATGTGTGCTTAAGCATGTGTACATTCCTCTCTTACCTATAATGGTACC-3′ (i.e. SEQ ID NO.163) were designed. Plasmid pP43NMK was used as a template and a plasmid fragment was obtained by reverse amplification by PCR. Finally, the recombinant plasmid was constructed by Gibson Assembly Clonging Kit (New England Biolabs), and it was verified that the construction of the recombinant pP43NMK-NO132-GFP plasmid was successful by sequencing.
(43) 2. Construction of Recombinant pP43NMK-NO138-GFP Plasmid Bacillus Subtilis
(44) The constructed pP43NMK-NO138-GFP plasmid was transformed into a wild type strain of Bacillus subtilis 168. Primers yz_zong-p43NMK_F: 5′-TTCTTGCTGAGTCTGGCTTTCG-3′ (i.e. SEQ ID NO.156) and yz_zong-p43NMK_R: 5′-CGGCTCGTATGTTGTGTGGAAT-3′ (i.e. SEQ ID NO.157) were used to select transformants for colony PCR, and it was verified that the construction of the recombinant Bacillus subtilis successful was when a 1.8 kb band appeared.
(45) 3. Expression of green fluorescent protein in engineering bacteria after addition of N-terminal sequence
(46) Seeds of successfully constructed recombinant Bacillus subtilis cultured at 37° C., 200 rpm for 10 h were transferred to the fermentation medium according to an inoculum size of 10% (v/v), and cultured at 37° C., 200 rpm for 20 h.
(47) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.18 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.131 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(48) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.33 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.132 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(49) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.29 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.133 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(50) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.34 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.134 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(51) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.39 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.135 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(52) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.41 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.136 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(53) Under the same conditions, if the original N-terminal sequence as shown in SEQ ID NO.76 is added, the final fluorescent intensity change curve is not coupled to growth; while after the N-terminal sequence element as shown in SEQ ID NO.137 is added, it was measured that the fluorescent intensity is coupled to growth, as shown in
(54) The N-terminal sequence elements as shown in SEQ ID NO.131-137 was respectively added to the N-terminal of the GFP nucleotide sequence of the protein of interest, to verify the effects on the expression of the protein. The results are shown in Table 6.
(55) TABLE-US-00006 TABLE 6 Increase of protein expression by addition of 7 artificially designed N-terminal sequence elements Fermentation time: 4 h 20 h Average Average N-terminal fluorescent fluorescent sequence number intensity Error Gain intensity Error Gain SEQ ID NO. 131 5004.60 200.75 0.97 19761.00 512.97 0.41 SEQ ID NO. 132 9422.25 276.65 1.83 50650.67 2052.89 1.05 SEQ ID NO. 133 11164.25 418.75 2.16 37814.25 1281.37 0.78 SEQ ID NO. 134 7152.60 120.61 1.39 29728.60 207.00 0.62 SEQ ID NO. 135 4700.60 190.81 0.91 19497.20 578.99 0.40 SEQ ID NO. 136 9504.50 427.54 1.84 30170.00 702.68 0.63 SEQ ID NO. 137 1916.80 124.38 0.37 5567.80 156.86 0.12
Comparative Example Construction of a Control Group Without Specific N-Terminal Sequence
(56) The composition of the recombinant control plasmid is that the green fluorescent protein (GFP) gene is directly inserted after the P43 promoter of the Pp43NMK plasmid. Primers rh_Ctr-0.75k_p43NMK-GFP_F: 5′-ACACATGAGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCA-3′ (i.e. SEQ ID NO.158), and rh_Ctr-0.75k_p43NMK-GFP_R: 5′-TACGCCAAGCTTTCATCACTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAG-3′ (i.e. SEQ ID NO.153) were designed, Escherichia coli containing the green fluorescent protein (GFP, GenBank: AF324408.1) gene was used as a template, and a green fluorescent protein fragment was obtained by colony PCR. Primers fx_ctr-6.7k_p43NMK-GFP_F: 5′-AGTGATGAAAGCTTGGCGTAATCATGGTCATAGCTGTTT-3′ (i.e. SEQ ID NO.154), and fx_ctr-6.7k_p43NMK-GFP_R: 5′-CTTCTCCTTTACTCATGTGTACATTCCTCTCTTACCTATAATGGTACCGCTATCACTT-3′ (i.e. SEQ ID NO. 164) were designed. Plasmid pP43NMK was used as a template and a plasmid fragment was obtained by reverse amplification by PCR. Finally, the recombinant plasmid by Gibson Assembly Clonging Kit (New England Biolabs) was constructed. After verifying that the construction of the recombinant pP43NMK-Ctr-GFP plasmid was successful by sequencing, a Bacillus subtilis 168 wild type was transformed. It was verified that the plasmid is successfully transformed by colony PCR.
(57) If transferring seeds of the recombinant Bacillus subtilis cultured at 37° C., 750 rpm in a 700 μL LB medium and in a 96-well deep-well plate for 9 h to a 190 μL LB medium according to an inoculum size of 5% (v/v) and culturing the seeds at 37° C., 750 rpm for 4 h or 20 h. Finally, the fluorescent intensity measured in the fermentation broth after 4 h is 5159, which is only 14% of the fluorescent intensity after addition of the N-terminal sequence (i.e. SEQ ID NO.18) of YdbP protein; the fluorescent intensity measured in the fermentation broth after 20 h is 48181, which is only 35% of the fluorescent intensity after addition of the N-terminal sequence of YdbP protein.
(58) Although the present disclosure has been disclosed above in the preferred examples, it is not intended to limit the present disclosure. Any modifications and variations can be made without departing from the spirit and scope of the present disclosure by any person skilled in the art, and the scope of the present disclosure shall be determined by the scope of the appended claims.