CN109504690B - Stress, signal and transcription regulation gene involved in regulating and controlling yield of streptomycete ACT - Google Patents

Stress, signal and transcription regulation gene involved in regulating and controlling yield of streptomycete ACT Download PDF

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CN109504690B
CN109504690B CN201910040557.0A CN201910040557A CN109504690B CN 109504690 B CN109504690 B CN 109504690B CN 201910040557 A CN201910040557 A CN 201910040557A CN 109504690 B CN109504690 B CN 109504690B
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徐钟
李远远
王永
王法云
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Henan Business Research Institute Co ltd
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Abstract

The application belongs to the technical field of microbial fermentation engineering, and particularly relates to a gene related to the yield of Actinorhodin (ACT) of a polyketide in streptomyces. The application specifically relates to the application of stress, signal and transcription regulation genes in the aspect of regulating and controlling the yield of the streptomycete ACT, wherein the number of the stress, signal and transcription regulation genes is 14; after the gene mutation, the gene has regulation and control influence on the yield of streptomyces ACT. The inventors have mutagenized Streptomyces coelicolor M145 and screened strains with altered actinorhodin production. The position of the transposon on the genome is positioned by the screened positive clones through enzyme digestion, self-ligation and sequencing, and the spontaneous mutant gene is eliminated by the principle of screening and positioning the same gene for a plurality of times, and finally the gene influencing the yield of the actinorhodin is determined.

Description

Stress, signal and transcription regulation gene involved in regulating and controlling yield of streptomycete ACT
Technical Field
The application belongs to the technical field of microbial fermentation engineering, and particularly relates to a gene related to the yield of Actinorhodin (ACT) of a polyketide in streptomyces.
Background
The existing research generally considers that small molecular compounds generated by the secondary metabolism of microorganisms have important significance on human health. Statistics indicate that more than 60% of the current FDA-approved anti-infective and anti-tumor drugs are derived from microbial secondary metabolites. As more and more genome sequencing work of microorganisms is carried out, genome sequence analysis shows that the microorganisms have great potential for generating various secondary metabolites, but partial research shows that many secondary metabolites of the microorganisms cannot be expressed under the laboratory culture condition, and most environmental microorganisms cannot be effectively cultured under the laboratory condition, so that the development of the secondary metabolites of the microorganisms is seriously hindered.
In the existing research, streptomyces is an important antibiotic producing bacterium, and the production of the antibiotic is controlled by environmental signals and self-regulating genes. The streptomyces coelicolor is a model strain for researching the differentiation and secondary metabolism of streptomyces and can produce two colored antibiotics actinorhodin (ACT blue) and undecylprodigiosin (Red Red), and ACT and RED synthetases belong to type I polyketide synthase (I-PKS) and type II polyketide synthase (II-PKS), respectively. The 2 secondary metabolites in the streptomyces coelicolor are taken as a model for researching the synthesis and regulation of the secondary metabolism of the streptomyces coelicolor, and aiming at the screening of the 2 secondary metabolite regulation genes, a good foundation can be laid for the genetic modification of antibiotic producing bacteria, the yield improvement of antibiotic industrial strains or the activation and expression of silent gene clusters.
In the prior art, the inventor uses transposition mutagenesis technology to research the functional genome of streptomyces coelicolor A3(2) in early stage and initially constructs a streptomyces coelicolor A (3)2 mutant library (specifically, refer to Xuzhong, research the functional genome of streptomyces coelicolor A3(2) by using transposition mutagenesis, 2011 university of Master thesis in Huazhong agriculture), but because of complexity and uncertainty of related gene regulation functions, further intensive research and discussion are needed for specific genes related to regulation of secondary metabolites.
Disclosure of Invention
The application aims to provide a part of genes related to ACT metabolic regulation in the microorganism, so as to lay a foundation for streptomycete secondary metabolite research and novel drug development.
The technical solution adopted in the present application is described in detail as follows.
Genes influencing the yield of ACT in streptomyces, wherein the genes have a regulation and control effect in the synthesis of a streptomyces polyketide ACT; examples of the microorganism include Streptomyces coelicolor (S. coelicolor)Streptomyces coelicolor) (ii) a The genes are classified into four major groups according to their existing gene annotation, specifically:
cells are synthesized in regulatory classes:
a total of 7 including genesSCO1525SCO2097SCO2132SCO3150SCO4440SCO4878SCO5174(ii) a According to the existing gene annotation, in particular:
SCO1525 and SCO2132 are involved in cell wall phosphatidylinositol mannosylation modification;
SCO2097 is involved in cell wall synthesis;
SCO3150 is involved in cell lysis;
SCO4440 is involved in cell membrane phosphatidylinositol signal regulation;
SCO4878 and SCO5174 are involved in cell wall glycosylation modification;
in the present application, after the mutation (gene deletion or inactivation) of the gene, the expression level (yield) of ACT is decreased, in other words, the gene has a positive regulation effect on the expression level (yield) of ACT; that is, after the gene is mutated (gene deletion or inactivation), the expression quantity (yield) of the ACT is reduced, and after the copy number of the gene is increased or the gene is over-expressed, the gene has the potential of regulating the expression quantity (yield) of the ACT;
amino acid metabolism classes:
7 in total; involving association with amino acid metabolismSCO2241SCO2528SCO3345SCO5281SCO5512SCO2999SCO3962(ii) a According to the existing gene annotation, in particular:
SCO2241 participates in the synthesis of glutamic acid;
SCO2528 is involved in leucine synthesis;
SCO3345 is involved in the synthesis of valine and isoleucine;
SCO5281 α -ketoglutarate decarboxylase;
SCO5512 is involved in branched amino acid metabolism;
the SCO2999 is involved in the metabolism of glutamic acid,
SCO3962 is involved in prephenate metabolism;
in the present application, after the mutation of the gene (gene deletion or inactivation), the gene has uncertain regulatory influence on ACT expression (yield), and further:
SCO2241SCO2528SCO3345SCO5281andSCO5512after any one of the 5 genes is mutated (gene deletion or inactivation), the expression level (yield) of ACT is reduced, in other words, the 5 genes have positive regulation effect; that is, any of these 5 genes, which regulates the decrease in the amount of ACT expression (yield) after mutation (gene deletion or inactivation), is usedAfter the copy number is increased or the copy number is over-expressed, the potential of regulating and controlling the increase of ACT expression quantity (yield) is realized;
SCO2999andSCO3962after any one of the 2 genes is mutated (gene deletion or inactivation), the expression level (yield) of ACT is increased, in other words, the 2 genes have a negative regulation effect; that is, any of the 2 genes can regulate the increase of the expression level (yield) of the ACT after mutation (gene deletion or inactivation), and the possibility of regulating the decrease of the expression level (yield) of the ACT can be realized after the copy number of the genes is increased or even the genes are over-expressed;
stress, signal and transcriptional regulation classes:
a total of 14, including genes:SCO0871SCO1663SCO2832SCO2987SCO3571SCO4204SCO4215SCO4358SCO6994SCO1728SCO2686SCO3008SCO5220SCO6636
according to the existing gene annotation, in particular:
the SCO0871 participates in the regulation of signals,
SCO1663, SCO4204 and SCO2987 participate in environmental stress regulation,
SCO2832, SCO3571, SCO4215, SCO4358, SCO6994, SCO1728, SCO2686, SCO3008, SCO5220 and SCO6636 are transcription regulation proteins;
in the present application, after the mutation of the gene (gene deletion or inactivation), the gene has uncertain regulatory influence on ACT expression (yield), and further:
SCO0871SCO1663SCO2832SCO2987SCO3571SCO4204SCO4215SCO4358andSCO6994after any one of the 9 genes is mutated (gene deletion or inactivation), the expression level (yield) of ACT is reduced, in other words, the 9 genes have positive regulation effect; that is, any of the 9 genes can regulate the ACT expression level (yield) to be reduced after mutation (gene deletion or inactivation), and can regulate the ACT expression level (yield) after the copy number of the gene is increased or over-expressed) Increased potential;
SCO1728SCO2686SCO3008SCO5220andSCO6636after any one of the 5 genes is mutated (gene deletion or inactivation), the expression level (yield) of ACT is increased, in other words, the 5 genes have negative regulation effect; that is, any of the 5 genes can regulate the increase of the expression level (yield) of the ACT after mutation (gene deletion or inactivation), and the regulation of the expression level (yield) of the ACT can be reduced after the genes are complemented back, copy number is increased or overexpressed;
transporters:
6 in total; the method comprises the following steps:SCO2254SCO2534SCO3765SCO6160SCO2519SCO3185(ii) a According to the existing gene annotation, in particular:
SCO2254 is a transmembrane channel protein;
SCO2534, SCO3765 and SCO3185 participate in ion transport;
SCO2519 is involved in lipid transport and antibiotic efflux;
SCO6160 is involved in protein transport;
in the present application, after the mutation of the gene (gene deletion or inactivation), the gene has uncertain regulation and control effects on ACT expression level (yield), and further:
SCO2254SCO2534SCO3765andSCO6160after any one of the 4 genes is mutated (gene deletion or inactivation), the expression level (yield) of ACT is reduced, in other words, the 4 genes have positive regulation effect; that is, any of the 4 genes can regulate the reduction of the expression level (yield) of ACT after mutation (gene deletion or inactivation), and has the potential of regulating the increase of the expression level (yield) of ACT after the copy number of the genes is increased or over-expressed;
SCO2519andSCO3185after any one of the 2 genes is mutated (gene deletion or inactivation), the expression level (yield) of ACT is increased, in other words, the 2 genes have a negative regulation effect; that is, any of these 2 genes is mutated (gene deletion orInactivation), the regulated ACT expression level (yield) is increased, and after the genes are complemented back, the copy number is increased or over-expressed, the regulated ACT expression level (yield) is possibly reduced.
In the application, in order to systematically excavate a series of genes influencing and controlling the yield of Actinorhodin (ACT) in an antibiotic-producing strain streptomyces coelicolor, the inventor adopts an in-vivo transposition system based on mini-Tn5 to mutate streptomyces coelicolor M145 and further screens strains with variable Actinorhodin yield. The experimental results show that: the vector (pHL 734) used in the mutagenesis system does not contain a Streptomyces replicon and an integration site, and only one transposition event can occur after the vector is transferred into a Streptomyces cell by conjugation, so that each positive clone genome screened only contains one randomly inserted mini-Tn5 copy. And further positioning the position of the transposon on the genome of the screened positive clone by enzyme digestion, self-ligation and sequencing, and eliminating a spontaneous mutant gene by the principle of repeatedly screening and positioning the same gene, thereby finally determining the gene influencing the yield of the actinorhodin. Further taking the wild type strain as a reference, and finally determining that the related genes influence the yield of the actinorhodin through fermentation culture. Based on the screening results, a foundation can be laid for the regulation of the yield of related metabolites or the synthesis of new secondary metabolites by further using a genetic engineering technical means.
Detailed Description
The present application is further illustrated by the following examples. Before describing the specific embodiments, a brief description will be given of some experimental background cases in the following embodiments.
Biological material:
streptomyces coelicolor M145 (Streptomyces coelicolor M145) (prototrophic wild type strain A3 (2)) as a transposable mutagenesis starting strain;
escherichia coli ET12567/pUZ8002 (Escherichia coliET12567/pUZ 8002) for introducing plasmid pHL734 into streptomyces coelicolor M145;
plasmid pHL734 carries transposable element Mini-Tn5 and transposase, and is used for transposable mutagenesis of Streptomyces coelicolor M145;
experimental reagent:
LB culture medium is used for culturing Escherichia coli at 37 ℃;
YEME culture medium and TSBY culture medium are used for culturing streptomycete liquid,
adding MgSO (MgSO) into SFM medium4(20 mM) for conjugal transfer of Streptomyces;
the YBP culture medium is used for streptomycete solid culture and fermentation, and the culture temperature of the streptomycete is 30 ℃;
apramycin (Apramycin, Apr), resistance geneAcc(3)IVThe use concentration is 50 mug/mL;
trimethoxybenzylaminopyrimidine (Trimethoprim, TMP) is used at a concentration of 50. mu.g/mL.
Example 1
This example is briefly described below with respect to the mutagenesis procedure of S.coelicolor M145 using the mini-Tn5 transposition system. It should be noted that the detailed process is described in "study of functional genome of Streptomyces coelicolor A3(2) by transposable mutagenesis" (Xuzhong, 2011 Master thesis at Huazhong university of agriculture).
Transposons transposable mutagenesis of Streptomyces coelicolor
Firstly, referring to the prior art, a transposon plasmid pHL734 is introduced into streptomycete by conjugal transfer of an escherichia coli strain ET12567/pUZ8002 and streptomyces coelicolor, and the ratio of recipient bacteria to donor bacteria is 1: 1;
theoretically, after entering the streptomycete, the transposase Tnp (5) starts to express, the mini-Tn5 fragment is cut and randomly inserted into the genome of the streptomycete, and the plasmid disappears after the transposition occurs because the plasmid cannot replicate and integrate sites in the streptomycete;
covering the cells with TMP and Apr (screening mutants with transposition insertion through an apramycin resistance gene inside Mini-Tn 5) about 12-14 hours after conjugation transfer, and culturing for about 4-5 days; the resulting conjugative transfer clones were transferred to YBP medium (each mutant contains a transposition insert) and mutants with varying secondary metabolite production were selected.
(II) transposition insertion mapping of mutant strains
Respectively extracting the total DNA of the mutant strain with the change of the secondary metabolite yield in the step (I), and carrying out enzyme digestion on the total DNA by using ApaI restriction enzyme;
introducing the digested DNA sample into escherichia coli DH5 alpha through self-ligation and chemical transformation;
screening clone containing mini-Tn5 fragment by using apramycin, sequencing to obtain genome sequences at two ends of mini-Tn5 and a transposition insertion site thereof, and positioning the position of the transposition insertion on a chromosome through sequence comparison.
(III) complementation of mutant strains
Selecting 5 genes related to transcription regulationSCO2832SCO4215SCO4358SCO2686AndSCO3008the back-supplementing verification is carried out,
CDS and upstream 250 bp promoter region sequences of the genes are amplified by PCR, are connected to a streptomycete integration vector pMT3, are transformed into Escherichia coli ET12567/pUZ8002 after being verified to be correct by sequencing, and are transferred into a streptomycete mutant strain through the conjugation of the Escherichia coli and the streptomycete;
after the genome of the 5-gene mutant strain is respectively introduced with corresponding normal gene copies, the actinorhodin yield is restored to the wild level, which shows that the regulation and control of the actinorhodin yield by the genes repeatedly screened for many times are 100 percent correct.
(IV) determination of ACT production by mutant strains
The transposable mutant and the original strain are respectively cultured in solid YBP for 84 hours at 30 ℃, and 0.5 g of each culture product is used for ACT yield determination; ACT yield determination:
0.5 mL of 1M NaOH was added to 0.5 g of the culture product, disrupted by a homogenizer (5,000 rpm, 15 s; twice), centrifuged (12000 Xg, 5 min) to take the supernatant, and the absorbance of the supernatant was measured by UV ray at 633 nm to obtain the relative yield of ACT of the Mutant strain (Mutant 633/WT 633).
Example 2
This example is briefly described below with respect to the screening results of example 1.
On the basis of the screening method of example 1, 988 strains with changed actinorhodin production were screened from 50000 mutants as a result, and the transposition insertion sites of the strains were located to show that the mutant strains relate to 551 genes; some of the genes having a regulatory effect on the production of actinorhodin are specifically explained below.
Cells are synthesized in regulatory classes:
a total of 7 including genesSCO1525SCO2097SCO2132SCO3150SCO4440SCO4878SCO5174
Figure DEST_PATH_IMAGE001
Note (the following tabular data are synonymous and will not be described): in the table, relative ACT production indicates the ratio of ACT production of mutant strain to that of wild type strain, less than 1 indicates that ACT production of mutant strain is reduced, 0 indicates that ACT production is not detected, and a plurality of values are indicated by "spaced apart" and indicate that a plurality of mutant strains of the same gene have different insertion sites of mini-Tn5 in the gene.
Note that, in the above table data, the annotation contents are obtained by integrating StrepDB data (http:// StrepDB. streptomyces. org. uk) and literature reports; ACT relative yields were calculated from the mean values for each mutant (data in the tables below are synonymous and are not described).
Analysis of the data in the above table shows that the actinorhodin production is reduced after 7 cells are inactivated by genes related to synthesis, which indicates that the integrity of the cell envelope is necessary for the synthesis of ACT, and the mutation (inactivation) of the genes has a positive correlation with the actinorhodin production.
Amino acid metabolism classes:
7 in total; involving association with amino acid metabolismSCO2241SCO2528SCO3345SCO5281SCO5512SCO2999SCO3962
Figure 289639DEST_PATH_IMAGE002
Analysis can see that:
SCO2241SCO2528SCO3345SCO5281andSCO5512all mutant strains of the gene had reduced ACT yield, indicating that the products encoded by these genes favor ACT synthesis,
whileSCO2999AndSCO3962all mutant strains of the genes showed elevated ACT production, indicating that the encoded products of these genes are detrimental to ACT synthesis.
Stress, signal and transcriptional regulation classes:
a total of 14, including genesSCO0871、SCO1663、SCO2832、SCO2987、SCO3571、SCO4204、 SCO4215、SCO4358、SCO6994、SCO1728、SCO2686、SCO3008、SCO5220、SCO6636
Figure DEST_PATH_IMAGE003
Analysis can see that:
SCO0871、SCO1663、SCO2832、SCO2987、SCO3571、SCO4204、SCO4215、SCO4358andSCO6994all mutant strains of the genes have reduced ACT yield, which indicates that the coded products of the genes are favorable for ACT synthesis;
SCO1728、SCO2686、SCO3008、SCO5220andSCO6636all mutant strains of the genes showed elevated ACT production, indicating that the encoded products of these genes are detrimental to ACT synthesis.
Transporters:
a total of 6, including genesSCO2254、SCO2534、SCO3765、SCO6160、SCO2519、SCO3185
Figure 255714DEST_PATH_IMAGE004
Analysis can see that:
SCO2254、SCO2534、SCO3765andSCO6160all mutant strains of the genes have reduced ACT yield, which indicates that the coded products of the genes are favorable for ACT synthesis;
SCO2519andSCO3185all mutant strains of the genes showed elevated ACT production, indicating that the encoded products of these genes are detrimental to ACT synthesis.
In conclusion, based on the effect of the different genes on the yield of ACT, one or more of the genes can be subjected to independent mutation or combined mutation to inactivate the genes, or overexpression is performed by using transgenic engineering, so that the yield of ACT is specifically regulated, and the production performance of antibiotics is further improved.

Claims (1)

1. The application of the transcription regulation and control gene in the aspect of regulating and controlling the yield of the streptomycete ACT is characterized in that the number of the transcription regulation and control genes is 10; the method comprises the following steps: SCO2832, SCO3571, SCO4215, SCO4358, SCO6994, SCO1728, SCO2686, SCO3008, SCO5220, SCO 6636;
after the gene mutation, the gene has regulation and control influence on the yield of streptomyces ACT;
the mutation is: a gene deletion or inactivating mutation;
the regulation and control influence is specifically as follows:
after any one of the 5 genes SCO2832, SCO3571, SCO4215, SCO4358 and SCO6994 is mutated, the ACT yield is reduced;
the ACT yield is increased after any one of 5 genes SCO1728, SCO2686, SCO3008, SCO5220 and SCO6636 is mutated;
the streptomyces is streptomyces coelicolor.
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Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN102212533A (en) * 2011-04-18 2011-10-12 河北农业大学 Negative regulator gene of streptomyces roseofulvus as well as preparation method and application thereof
CN103881951A (en) * 2014-03-26 2014-06-25 中国科学院微生物研究所 SCO6974 gene deleted streptomyces coelicolor and application thereof to yield increment of antibiotics

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EP1818398A1 (en) * 2006-02-14 2007-08-15 Universiteit Leiden Methods and means for metabolic engineering and improved product formation by micro-organisms

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CN102212533A (en) * 2011-04-18 2011-10-12 河北农业大学 Negative regulator gene of streptomyces roseofulvus as well as preparation method and application thereof
CN103881951A (en) * 2014-03-26 2014-06-25 中国科学院微生物研究所 SCO6974 gene deleted streptomyces coelicolor and application thereof to yield increment of antibiotics

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