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    • 专利摘要:
    The present application relates to improved yeast strains of Saccharomyces cerevisiae, characterized in that they coexpress a gene encoding a glucoamylase of fungal origin and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus. The present invention also relates to a method for obtaining these yeast strains, said method comprising the following steps: a) genetic modification of a yeast of Saccharomyces cerevisiae so as to co-express a gene encoding a glucoamylase of origin fungal and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus; b) culturing and fermentation of the strain obtained in step a) on a dextrin medium; c) selection of strains exhibiting fermentation kinetics at least equal to or greater than the strain deposited on 9 July 2015 under the Budapest Treaty to the CNCM under number I-4999 under the same conditions. The yeast strains according to the invention are of particular interest in the production of bioethanol.
    公开号:FR3040395A1
    申请号:FR1558079
    申请日:2015-08-31
    公开日:2017-03-03
    发明作者:Maud Petit;Georges Pignede;Jean-Michel Bavouzet;Benoit Thomas
    申请人:Lesaffre et Cie SA;
    IPC主号:
    专利说明:

    YEAST STRAINS CO-EXPRESSING EXOGENOUS GLUCOAMYLASES, PROCESS FOR OBTAINING THEM AND USE THEREOF FOR PRODUCING
    BIOETHANOL
    Technical field of the invention
    The present invention relates to Saccharomyces cerevisiae yeast strains genetically engineered to co-express genes encoding fungal glucoamylases and Saccharomyces cerevisiae var. diastaticus. Such strains are particularly interesting in the production of biofuel, especially bioethanol. The present invention also relates to a process for obtaining these yeasts as well as the use of these yeasts to produce bioethanol.
    BACKGROUND The use of biomass for bioethanol production has attracted considerable interest in recent years. Ethanol produced from agricultural residues, industrial waste and fast-growing plants has been proposed as a promising alternative fuel.
    Currently, the so-called first-generation bioethanol is produced mainly from cane sugar and starch-rich grains in Brazil and the United States respectively, using Saccharomyces cerevisiae yeast strains, which ferment glucose to ethanol with alcoholic strength, productivity and high efficiency.
    The process of converting starch into bioethanol requires prehydrolysis and liquefaction of biomass starch, conversion of liquefied starch to fermentable sugars (by hydrolysis of starch) and fermentation of these sugars to ethanol . These last two steps are often performed simultaneously. The hydrolysis of starch requires the action of so-called amylolytic enzymes, but, unfortunately, S. cerevisiae is devoid of this type of enzymes. Currently, the production of ethanol from the biomass composed of starch therefore requires the addition of exogenous enzymes in two steps: a first step of addition of exogenous amylolytic enzymes so as to pre-hydrolyze and liquefy the starch contained in biomass; and a second step wherein other exogenous enzymes are used to hydrolyze liquefied starch and a yeast strain of S. cerevisiae to ferment the fermentable sugars released. The use of exogenous enzymes leads to significant costs and time losses, and it would therefore be very advantageous to obtain yeast strains which are both capable of hydrolyzing liquefied starch while being capable of to effectively ferment the sugars resulting from the hydrolysis of liquefied starch.
    Invention
    In this context, the inventors of the present invention have developed a genetically modified strain of Saccharomyces cerevisiae, said strain co-expressing several exogenous glucoamylase genes. In particular, the strains of Saccharomyces cerevisiae according to the invention co-express both a gene encoding a glucoamylase of fungal origin and a gene coding for the glucoamylase of Saccharomyces cerevisiae var. diastaticus. The inventors have demonstrated that these strains are capable of hydrolyzing liquefied starch extracted from biomass while succeeding in effectively fermenting the sugars resulting from this hydrolysis. Indeed, the use of a yeast strain according to the present invention makes it possible to replace all or part of the amount of exogenous enzymes required during the conversion of liquefied starch into bioethanol.
    Thus, according to a first aspect, the present invention relates to a yeast strain of Saccharomyces cerevisiae, characterized in that it coexpresses: a gene encoding a glucoamylase of fungal origin; and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus.
    The inventors have also developed a method for obtaining strains of Saccharomyces cerevisiae having the ability to both hydrolyze starch and ferment the sugars resulting from this hydrolysis.
    Thus, according to a second aspect, the present invention relates to a method for obtaining a yeast strain, said method comprising the following steps: a) genetic modification of a yeast of Saccharomyces cerevisiae so as to make it express a coding gene a glucoamylase of fungal origin and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus; b) culturing and fermentation of the strain obtained in step a) on a dextrin medium; c) selection of strains exhibiting fermentation kinetics at least equal to or greater than that obtained with the strain deposited on 9 July 2015 under the Budapest Treaty to the CNCM under number 1-4999 under the same conditions.
    According to another aspect, the present invention relates to a process for producing bioethanol from a biomass characterized in that it comprises the following steps: a) prehydrolysis and liquefaction of the starch of the biomass; b) bringing the liquefied starch obtained in step a) into contact with a modified Saccharomyces cerevisiae yeast according to the invention; c) hydrolysis and fermentation of the liquefied starch by said yeast; d) extracting the ethanol produced in step c).
    In addition, the present invention relates to the use of a modified yeast strain Saccharomyces cerevisiae according to the invention for the production of biofuel.
    Detailed description of the invention
    In order to obtain a yeast strain that can hydrolyze the starch and ferment the sugars resulting from the hydrolysis of the starch, the inventors have genetically modified a strain of Saccharomyces cerevisiae so as to make it co-express two genes coding for exogenous glucoamylases.
    Thus, a first subject of the present invention is a yeast strain of Saccharomyces cerevisiae, characterized in that it expresses: a gene encoding a glucoamylase of fungal origin; and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus.
    In particular, the subject of the present invention is a yeast strain of Saccharomyces cerevisiae, characterized in that it expresses: a gene encoding a glucoamylase of fungal origin; and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus in which the glucoamylase of Saccharomyces cerevisiae var. diastaticus has the protein sequence SEQ ID NO: 4.
    Surprisingly, the inventors have discovered that the specific use of a glucoamylase gene of Saccharomyces cerevisiae var. diastaticus and a glucoamylase gene of fungal origin provided strains with excellent hydrolysis capabilities.
    These results are particularly surprising, since the glucoamylase of Saccharomyces cerevisiae var. diastaticus is known to have a much less efficient yield than that obtained with glucoamylases of fungal origin, making it an enzyme very little used by enzymiers. This postulate is for example demonstrated in the international patent application published under the reference WO2011 / 153516, which describes the screening enzymes whose glucoamylase Saccharomyces cerevisiae var. diastaticus (which corresponds to the protein IDAAA35107.1). In this document, the glucoamylase of Saccharomyces cerevisiae var. diastaticus is not considered interesting for its enzymatic activity. The term "yeast strain" refers to a relatively homogeneous population of yeast cells. A yeast strain is obtained from a clone, a clone being a cell population obtained from a single yeast cell.
    By "gene encoding glucoamylase" is meant herein an amino acid sequence which, when expressed, will provide a functional glucoamylase protein.
    By "glucoamylase" is meant herein an enzyme capable of hydrolyzing α-1,4 glycosidic linkages of crude or soluble starch from the non-reducing end of amylose and amylopectin. Amylases are also known as amyloglucosidases or γ-amylases (MEDLINE referenced: EC 3.2.1.3). In addition to acting on the α-1,4 bonds, the glucoamylase enzyme can slowly hydrolyze the α-1,6 bonds of the amylopectin molecules, provided that the neighboring link in the sequence is an α-1 bond, 4.
    A glucoamylase of fungal origin is chosen from commercial glucoamylases known for their good enzymatic activity and, in particular, the glucoamylase of fungal origin is selected from the group consisting of: an Aspergillus niger glucoamylase, a glucoamylase of Saccharomycopsis fibuligera, Trichoderma reesei glucoamylase, Rhizopus oryzae glucoamylase, Aspergillus oryzae glucoamylase and Thermomyces lanuginosis glucoamylase.
    These glucoamylases are known to those skilled in the art, and their sequences are accessible under the references GenBank (http://www.ncbi.nlm.nih.gov/genha.nkA):
    Trichoderma reesei 4 ETS06561
    Rhizopus oryzae + BAA00033
    Aspergillus oryzae 4 BAA00841
    Thermomyces lanuginosis ABQ23180
    According to a particular embodiment, the glucoamylase of fungal origin is a glucoamylase with "Aspergillus niger or Saccharomycopsis fibuligera.
    The glucoamylase of Saccharomycopsis fibuligera is encoded by the GLU0111 gene which has the nucleic sequence corresponding to SEQ ID NO: 17 and has the sequence for protein sequence corresponding to SEQ ID NO: 18. The Aspergillus niger glucoamylase is coded by the GLAA gene which has the nucleic acid sequence corresponding to SEQ ID NO: 1 and has for protein sequence the sequence corresponding to SEQ ID NO: 2.
    The glucoamylase of Saccharomyces cerevisiae var. diastaticus is encoded by the STA1 gene which has the nucleic acid sequence corresponding to SEQ ID NO: 3 and has as a protein sequence the sequence corresponding to SEQ ID NO: 4.
    Thus, in a particular embodiment, the subject of the present invention is a yeast strain of Saccharomyces cerevisiae, characterized in that it contains the nucleic sequence SEQ ID NO: 1 and the nucleic sequence SEQ ID NO: 3.
    In one embodiment, the subject of the present invention is a yeast strain of Saccharomyces cerevisiae, characterized in that it co-expresses: a gene encoding Aspergillus niger glucoamylase; and a gene encoding Saccharomyces glucoamylase. cerevisiae var. diastaticus.
    In a particular embodiment, the invention relates to a yeast strain of Saccharomyces cerevisiae, characterized in that it co-expresses: a gene encoding Aspergillus niger glucoamylase; and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus where the glucoamylase of Saccharomyces cerevisiae var. diastaticus has the protein sequence SEQ ID NO: 4 and the Aspergillus niger glucoamylase has the protein sequence SEQ ID NO: 2.
    The terms "glucoamylase of fungal origin" and "glucoamylase of Saccharomyces cerevisiae var. diastaticus' should not be interpreted strictly: they include fungal glucoamylases and Saccharomyces cerevisiae var. diastaticus which are encoded by the nucleic sequences as described above, but also the functional variants of these glucoamylases.
    Typically, a functional variant of a glucoamylase according to the invention has a protein sequence having an identity percentage of at least 80%, 90%, 95%, more particularly 99% with the protein sequence of said glucoamylase. For example, functional variants of Aspergillus niger glucoamylases and Saccharomyces cerevisiae var. diastaticus have a protein sequence having an identity percentage of at least 80%, 90%, 95%, more particularly 99% respectively with the sequence SEQ ID NO: 2 or 4.
    The "percentage identity" is a comparison between amino acid sequences, and is determined by comparing two sequences aligned optimally on a comparison window. The skilled person knows how to calculate a percentage of identity between two sequences and has many tools allowing it. One of the two sequences may have amino acid deletions, insertions, and deletions with respect to the other sequence. Those skilled in the art will know how to select functional variants of glucoamylases according to inventkm. By "functional variant" is meant a variant which retains its glucoamylase activity and with similar kinetics of hydrolysis of starch. Methods for measuring and comparing kinetics of starch hydrolysis are described in the experimental part of the present application. Functional variants can be prepared by various conventional methods, such as, for example, random mutagenesis or site-directed mutagenesis. Those skilled in the art know multiple methods for introducing a gene into a yeast strain, in particular via the use of vectors comprising expression cassettes. By "vector" is meant any DNA sequence in which it is possible to insert foreign nucleic acid fragments, the vectors for introducing foreign DNA into a host cell. Examples of vectors are plasmids, cosmids, vectors derived from viruses. The vectors allow either the integration of heterologous genes directly into the yeast genome, or their expression in an independent plasmid. The introduction of vectors into a host cell is a method widely known to those skilled in the art. Several methods are described in particular in "Current Protocols in Molecular Biology", 13.7.1-13.7.10; or in Ellis T et al., Integrative Biology, 2011, 3 (2), 109-118.
    According to the invention, the gene encoding a glucoamylase of fungal origin and that encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus can be inserted within a single vector, or within two separate vectors.
    Thus, according to a particular aspect of the invention, the gene encoding a glucoamylase of fungal origin and that encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus are each separately integrated into a vector. According to a particular embodiment, the vector is a plasmid.
    In a particular embodiment of the invention, the gene encoding a glucoamylase of fungal origin and that encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus are integrated within the genome of said yeast.
    The vector according to the invention may also carry a selection marker. By "selection marker" is meant a gene whose expression gives the yeasts which contain it a characteristic enabling them to be selected. This is for example an antibiotic resistance gene or a gene for the growth of yeast on a particular medium.
    The genes according to the invention may be operably linked to a promoter, a terminator or any other sequence necessary for its expression in yeast.
    In a particular embodiment of the invention, the expression of the genes coding for glucoamylases of fungal origin and of Saccharomyces cerevisiae var. diastaticus is controlled by a so-called "strong" promoter. The skilled person knows the meaning of strong promoter. A strong promoter is for example the pADH1 promoter, the pTEF promoter, or the pTDH3 promoter.
    Thus, in one embodiment, the present invention relates to a yeast strain of Saccharomyces cerevisiae as described above, wherein the expression of the gene encoding a glucoamylase of fungal origin and that encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus is controlled by the pADH1 promoter.
    The genes encoding glucoamylases of fungal origin and Saccharomyces cerevisiae var. diastaticus may be present in several copies.
    Thus, in a particular embodiment, the present invention relates to a yeast strain of Saccharomyces cerevisiae as described above, characterized in that it comprises m copies of the gene encoding a glucoamylase of fungal origin and n copies of the gene. encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus, where m is an integer from 2 to 10 and n is an integer from 2 to 10. m and n are therefore independently 2, 3, 4, 5, 6, 7, 8, 9 or 10
    In a more particular embodiment, m is an integer between 2 and 8, and n is an integer between 2 and 8. The invention particularly relates to two yeast strains of Saccharomyces cerevisiae as described above, said strains being the strain deposited on 6 August 2015 under the Budapest Treaty to the CNCM under the number 1-5005 or the strain deposited on 9 July 2015 under the Budapest Treaty to the CNCM under the number 1-4997.
    Yeast strain 1-5005 comprises 4 copies of the gene encoding Aspergillus niger glucoamylase and 3 copies of the gene encoding Saccharomyces cerevisiae var glucoamylase. diastaticus.
    Yeast strain 1-4997 comprises 4 copies of the gene encoding Aspergillus niger glucoamylase and 4 copies of the gene encoding Saccharomyces cerevisiae var glucoamylase. diastaticus.
    The inventors have at the same time developed a method for obtaining strains of Saccharomyces cerevisiae which are capable of hydrolyzing starch.
    Thus, according to another aspect, the subject of the present invention is a method for obtaining a yeast strain, said method comprising the following steps: a) genetic modification of a yeast of Saccharomyces cerevisiae so as to make it to express a gene encoding a glucoamylase of fungal origin and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus; b) culturing and fermentation of the strain obtained in step a) on a dextrin medium; c) selection of strains exhibiting fermentation kinetics at least equal to or greater than that obtained with the reference strain deposited on 9 July 2015 under the Budapest Treaty to the CNCM under number 1-4999 under the same conditions.
    The yeast Saccharomyces cerevisiae of step a) is a yeast used for the production of bioethanol.
    According to a particular embodiment of the invention, the yeast Saccharomyces cerevisiae of step a) is the yeast Ethanol Red ®, hereinafter named ER, deposited at the CNCM on September 4, 2008 under the number 1-4071.
    By "dextrin medium" is meant a synthetic medium containing dextrins as known to those skilled in the art. This is for example a synthetic medium containing starch dextrins (220 g / kg), yeast extract (5 g / kg), urea (2 g / kg), dihydrogenphosphate of potassium (1 g / kg) as well as minerals and vitamins.
    The reference strain 1-4999 corresponds to the genetically modified strain of Ethanol Red ® yeast comprising 4 copies of the gene coding for the glucoamylase of
    Saccharomycopsis fibuligera.
    The kinetics of fermentation can be easily measured by various techniques known to those skilled in the art. For example, the kinetics of fermentation can be measured via a fermentation monitoring by weighing over time.
    The strains thus selected are particularly interesting for producing biofuel, in particular bioethanol from biomass.
    The term "biomass" refers to a set of organic materials that can be converted into energy. Many types of biomass, including wood, agricultural residues, herbaceous crops, can be used for the production of biofuel, particularly bioethanol. Bioethanol is characterized by "bio" because it is produced from renewable biomass.
    Thus, the present invention relates to a process for producing bioethanol from a biomass characterized in that it comprises the following steps: a) prehydrolysis and liquefaction of the starch of the biomass; b) bringing the liquefied starch obtained in step a) into contact with a yeast according to the invention; c) hydrolysis and fermentation of the liquefied starch by said yeast; d) extracting the ethanol produced in step c).
    According to a particular embodiment, the bioethanol production process described above further comprises a step b ') of adding exogenous glucoamylase enzymes after step b) and / or during step c) . The ethanol thus produced can have multiple uses, particularly in the automotive industry. The invention also relates to the use of a yeast strain as described above for the production of biofuel, particularly bioethanol.
    Brief description of the figures
    Figure 1 illustrates two examples of pANG and pSDG vectors for overexpression and cloning for glucoamylases. This vector is an integrative cloning vector used for the expression of genes in yeast. pADH1: S. cerevisiae ADH1 promoter; tCYCl: S. cerevisiae CYC1 terminator; Kan-MX: resistance marker to geneticin;
    AmpR: ampicillin resistance marker. BUD5 A and BUD5 B recombinogenic regions for integration at BUD5 locus.
    Figure 2 describes the cloning strategy for the insertion of 4 expression modules and a selection module at the HO locus.
    Figure 3 describes the strategy and the different steps for obtaining strains 1-5005 (A) and 1-4997 (B).
    FIG. 4 illustrates an exemplary result of screening of 88 ER-GAND clones on a YEG / starch medium. After 48 hours of incubation, the hydrolysis of the starch appears as clear halos around the yeast colonies secreting functional glucoamylases. Yeasts 1 to 6 on the 12th column are control strains allowing a comparison of the size and the intensity of the halos.
    FIG. 5 illustrates the screening carried out with the ER-GAND series 8000 clones in fermentation on dextrin medium. Three fermentation times (20h, 31h and 54h) are presented. The arrows indicate the 15 selected ER-GAND-series 8000 clones.
    Figure 6 shows dextrin fermentation of the best screened ER-GAND clones as well as 4 control strains (ER, 1-4998, 1-4899 and 1-4999). The fermentation is carried out at 32 ° C and is followed by loss of mass (g / kg) for 74h.
    Figure 7 shows a fermentation on corn industrial medium of the best screened ER-GAND 7000 clones as well as 3 control strains (1-4998, 1-4899 and 1-4999). The fermentation is carried out at 32 ° C and is followed by a loss of mass (g / kg) for 70h.
    EXAMPLES
    Example 1: Integration of 4 copies of the gene coding for Aspergillus niger glucoamylase and 3 or 4 copies of the gene coding for the glucoamylase of Saccharomyces cerevisiae var. diastaticus in a yeast strain of Saccharomyces cerevisiae
    The copies of Aspergilus niger GLAA (SEQ ID NO: 1) glucoamylase genes and S. cerevisiae var. STA1 diastaticus (SEQ ID NO: 3) were synthesized via codon for Saccharomyces cerevisiae.
    The DNA sequences used were cloned in a vector-type comprising: - the integration targets - the selected promoters / terminators, for example pADH1 / tCYC1 - the resistance markers that can be eliminated later.
    In the present example, the plasmid pANG (name internal to the applicant) was used to express the GLAA glucoamylase of Aspergillus niger (see FIG. In the same way, the plasmid pSDG (internal name to the applicant) is made to express the glucoamylase of S. cerevisiae var. diastaticus
    The principle of cloning 4 copies of GLAA or 3 or 4 copies STA1 can be detailed as follows: an expression module comprising the pADH1 promoter, the ORF of glucoamylases and the tCYCl terminator was amplified with 3 or 4 couples of different oligonucleotides. Each module obtained after PCR amplification has in common these 3 elements - A selection module comprising a strong promoter / terminator, a gene whose expression confers on the yeasts which contain it a characteristic enabling them to be selected. This is for example an antibiotic resistance gene or a gene for the growth of yeast on a particular medium. The antibiotic marker resistance module being flanked by LoxP sites, it will be possible to eliminate it a posteriori by action of Cre recombinase. "ORF" means "Open Reading Frame" meaning open reading frame.
    The primers used for the integration of the 4 copies of the GLAA gene and the selection module at the HO locus are as follows:
    If-Gibson AM G: TCTGATGGCTAACGGTGAAATTAAAGACATCGCAAACGTCACGGCTAACTTGAAGCTTCGTACGCTGCAGG (SEQ ID NO: 5)
    Al-Gibson AM G: TCACTGTACGGTGAGAACGTAGATGGTGTG CGCATAGGCCACTAGTGGATCT (SEQ ID NO: 6) A2-Gibson AMG: CACACC AT CT ACGTTCT CACCGT AC AGT GA GCATAACCGCTAGAGTACTT (SEQ ID NO: 7)
    Bl-Gibson AMG: TTACGTAGACTGAGTAGCAACGGTTGAGGA CAGCTTGCAAATTAAAGCCT (SEQ ID NO: 8) B2-Gibson AMG: TCCTCAACCGTTGCTACTCAGTCTACGTAA GCATAACCGCTAGAGTACTT (SEQ ID NO: 9)
    Cl-Gibson AMG: TCAGTAGCACAGAGAAGTGTAGGAGTGTAG CAGCTTGCAAATTAAAGCCT (SEQ ID NO: 10) C2-Gibson AMG: CT AC ACT CCT AC CTTTGTG CTTTG AT GCATAACCGCTAGAGTACTT (SEQ ID NO: 11)
    Dl-Gibson AMG: TTAGGATACATGCAGTAGACGAGGTAAGCA CAGCTTGCAAATT AAAGCCT (SEQ ID NO: 12) D2-Gibson AMG: TG CTTACCTCGTCTACTG CAT GTATCCTAA GC AT AACCGCTAG AGT ACTT (SEQ ID NO: 13) 2r-Gibson AMG: ACATACTTGCAATTTAT ACAGT GATG ACCGCTG AATTT GT AT CTT CCATACAGCTTGCAAATT AAAGCCT (SEQ ID NO: 14)
    The primers used for the integration of 3 or 4 copies of the STA1 gene and the selection module at the GRE3 locus are as follows: MCI-pADH1-GRE3-f:
    TAAGGGATATAGAAGCAAATAGTTGTCAGTGCAATCCTTCAAGACGATTG G CAT ACCG CTAG AGT ACTT (SEQ ID NO: 15)
    Al-Gibson AMG: T C ACT GTACGGT G AG AACGT AG ATGGT GT G CGCATAGGCCACTAGTGGATCT (SEQ ID NO: 6) A2-Gibson AMG: CACACC AT CTACGTTTC CACCGTACAGT GAAGGATATACCACCAGCTAG AGT ACTT (SEQ ID NO: 7)
    Bl-Gibson AMG: TT ACGTAG ACT G AGT AGCAACGGTT G AGG AT CAGCTTGCAAATTAAAGCCT (SEQ ID NO: 8) B2-Gibson AMG: TCCTCAACCGTTGCTACTCAGTCTACGTAA GCATAACCGCTAG AGT ACTT (SEQ ID NO: 9)
    Cl-Gibson AMG: TCAGTAGCACAGAGAAGTGTAGGAGTGTAG C AG CTT G CA AATT AAAGCCT (SEQ ID NO: 10) C2-Gibson AMG: CT AC ACT CCT AC CTTTGTG CTTTG TO GCATAACCGCTAGAGTACTT (SEQ ID NO: 11)
    Dl-Gibson AMG: TTAGGATACATGCAGTAGACGAGGTAAGCA CAGCTTGCAAATT AAAGCCT (SEQ ID NO: 12) D2-Gibson AMG: T G CTT ACCTCGTCTACTG CAT GTATCCTA A GCATAACCGCTAGAGTACTT (SEQ ID NO: 13) MCI-tCYCl-GRE3-r:
    CAC AT ATAC AG CAT G ATG AG AT ATGGAGGTTGAGT C G ATTT G AT ATGGGGGGGT G ATAG AGG G AT AGGAGG (SEQ ID NO: 16)
    Table 1 mentions the pairs of oligonucleotides used in the selection and expression modules.
    Table 1: Primer pairs used for cloning 4 copies of GLAA and 3 or 4 copies of ST Al "ANG gene" means Aspergillus niger glucoamylase gene. "SDG gene" means Saccharomyces cerevisiae var. Glucoamylase gene. diastaticus
    Each amplified module has recombinogenic sequences (Al, Bl, Cl and Dl) on either side of its promoter and its terminator. These sequences are provided by the floating tails of the PCR primers and will allow the modules to align and recombine specifically by homology between these recombinogenic sequences (FIG. 2).
    The strategy employed is to simultaneously integrate multiple expression modules of the glucoamylase genes into a S. cerevisiae strain in a single step at a given locus, based on the natural ability of the yeast to perform homologous recombination in vivo.
    Depending on the combinations of PCR products prepared, three or four glucoamylase expression modules and a selection module can be transformed into the S. cerevisiae strain.
    The selection of the clones having correctly integrated the expression cassettes is made initially on the basis of the presence of the selection module in the integration cassette (MCI).
    The presence of homologous sequences at a given locus, for example the HO locus, at the 5 'and 3' ends of the multi-integrative expression cassette allows the simultaneous integration of the expression modules and the selection module by homologous recombination. at this given locus. The use of different selection markers and their recycling as well as the integration at different loci allows the sequential and iterative integration of several multi-integrative cassettes.
    For example, FIG. 3 illustrates the various steps for obtaining the 1-4997 and I-5005 strains as explained below: 1- integration of 4 expression modules of the glucoamylase of A. niger, hereinafter GLAA, and the selection module G418 (geneticin resistance gene / KanMX marker) at the HO locus then making it possible to obtain the ER-ANG-G418 strain; 2- elimination of the selection module by the action of Cre recombinase allowing the selection of the strain deposited on October 15, 2014 at the CNCM under number 1-4899 5 3- integration of a second cassette composed of 3 or 4 modules of expression of the glucoamylase of S. cerevisiae var. diastaticus, hereinafter STA1, at the GRE3 locus.
    The strains expressing the glucoamylases of A. niger (GLAA) and S. diastaticus (STA1) were named ER-GAND. According to this construction model, it is thus possible to construct yeasts having integrated 4 copies of the GLAA glucoamylase gene and 3 copies of the STA1 glucoamylase gene or having integrated 4 copies of the GLAA glucoamylase gene and 4 copies of the STA1 glucoamylase gene.
    For ER-GAND yeasts two sets of clones were generated. The 7000 series (ER-GAND-7200 to ER-GAND-7376) corresponds to the integration of 4 copies of the glucoamylase GLAA gene (from Æ niger) and 3 copies of the STA1 glucoamylase gene (from S. cerevisiae var. diastaticus). As for the 8000 series (ER-GAND-8000 to ER-GAND-8159), 4 copies of the GLAA glucoamylase gene (from A. niger) and 4 copies of the ST al glucoamylase gene (from S. cerevisiae var. ) have been cloned.
    The yeast strains used in the invention are recalled below in Table 2 as well as their characteristics.
    Table 2: Summary of stem names / numbers and copy number of integrated glucoamylase genes (nd: not filed)
    Example 2: Screening of the strains
    Three phenotypic screens were carried out in order to select the fifteen best performing clones for the intended application. a) Phenotypic Screening with Iodine Hydrolysis of the soluble starch by the yeast transformants is tested on a YEG / starch agar medium (1% Glucose, 0.5% yeast extract, 1% soluble starch). The yeast cells are deposited on the YEG / starch agar and incubated for 2 days at 30 ° C. Then the boxes are stained with iodine vapor to visualize the hydrolysis halos present around the yeast colonies.
    This iodine vapor screening makes it possible to select clones secreting at least one enzyme capable of hydrolyzing starch. These positive clones can be visualized in particular by hydrolysis halos whose size is proportional to the enzymatic activity. FIG. 4 illustrates an example of screening of 88 ER-GAND clones on YEG medium / starch after iodine staining. Table 3 presents the results obtained after staining with iodine.
    Table 3: Results of the iodine screen for the 2 ER-GAND series.
    On 176 clones screened for each series, less than 3% of the clones tested do not seem to be able to hydrolyze the starch under the culture conditions of the example. Note that the host strain used in this strategy already had several glucoamylase genes in its genome, so a hydrolysis halo is present for this strain. These "negative" clones seem to have lost their glucoamylase genes. b) Phenotypic screening in fermentation in 0.5 g medium.
    The phenotypic screening on a dextrin medium under fermentation conditions makes it possible to eliminate the ER-GAND clones that can not ferment or ferment more slowly than the 1-4899 strain. For this, a visual monitoring of the biomass during the fermentation is carried out twice a day for 3 days. By comparing the rate of appearance of the biomass pellet with the 1-4999 and 1-4998 control strains, the most promising strains can then be selected.
    The ER-SDG-1c strain mentioned in the controls of FIG. 5 is an ethanol red ® strain expressing a copy of the S. diastaticus glucoamylase gene (STA1).
    The GO-ANG-4c strain mentioned in the controls of FIG. 5 is a GenOne + ® strain deposited at the CNCM on July 25, 2013 under the number 1-4791 expressing four copies of the A glucoamylase gene. Niger (GLAA)
    The fermentation medium used, the dextrin medium, is a synthetic medium containing starch dextrins (220 g / kg), yeast extract (5 g / kg), urea (2 g / kg) , KH2PO4 (1 g / kg) as well as minerals and vitamins. The fastest fermenting strains are strains capable of secreting a large amount of glucoamylase which then makes it possible to release glucose by hydrolysis of the dextrin molecules. The glucose thus released is then metabolized by the yeast S. cerevisiae to produce ethanol.
    Figure 5 illustrates an example of plate fermentation for the 88 ER-GAND clones. The pellets of biomass correspond to a fermentation of 31 h in dextrin medium. Clones indicated by an arrow have a higher biomass pellet than for strain I-4899. It is these clones that have been selected to be tested during fermentation on 100 g of dextrin medium.
    For each ER-GAND series, fifteen clones have been selected and will be tested during fermentation on 100 g of dextrin medium. c) Phenotypic screening in fermentation in a medium of 100 g.
    Fermentation on 100 g of selective synthetic dextrin medium (corn dextrin 220 g / kg, yeast extract 5 g / kg, urea 2 g / kg, KH 2 PO 4 1 g / kg as well as minerals and vitamins) is carried out at 32 g. ° C. Dextrins are starch hydrolysates to mimic the real environment.
    The S. cerevisiae strains modified according to the invention were previously propagated on YPG (Yeast extract, Peptone, Glucose) medium for 24 hours at 30 ° C. The initial pH of the fermentation medium was adjusted to 5.0 without regulation. The fermentation medium was then inoculated at a rate of 0.125 g dry matter equivalent per kilogram of medium. No exogenous hydrolysis enzyme is added to the fermentation medium. A loss of mass monitoring was carried out for 72 hours and is illustrated in FIG.
    In this type of fermentation medium (dextrin), there is little free glucose at 10 (about ten grams). The ER strain, having no enzyme capable of hydrolyzing dextrins, it consumes only available glucose and therefore a low mass loss is measured (about 5 g / kg). From the results of mass loss monitoring shown in FIG. 6, out of 30 clones tested, 3 groups can be established according to their kinetic fermentation behavior: Group A: 4 clones have a kinetic profile identical to the parent yeast strain I-4899 . - Group B: 2 clones have a kinetic profile similar to the reference strain I-4999 - Group C: the performance in fermentation kinetics of 24 clones is greater than that of the 1-4999 strain (target performance)
    Among the Group C strains, the 5 best clones of each series (series 7000 and 8000) were selected for testing on an industrial environment under real conditions of biofuel production.
    Example 3 Evaluation of the Production of Enzymatic Activity of Strains
    The ER-GAND clones with 4 copies of GLAA and 3 copies of STA1 (series 7000) selected previously, were evaluated at 32 ° C on the industrial medium E140723-11 and compared with the control strains 1-4998, 1- 4999 and 1-4899. These clones are: 7215, 7250, 7271, 7296, 7302. Clone 7302 corresponds to strain 1-5005.
    The strain (filed July 9, 2015 at the CNCM under number 1-4998) expressing STA1 activity from S. cerevisiae var. diastaticus made it possible to obtain rapid but incomplete dextrin hydrolysis kinetics, whereas the strain (1-4899) expressing the GLAA activity from A. niger made it possible to obtain a satisfactory hydrolysis of dextrins but with a lower kinetics of 1-4998.
    The strains were previously propagated on a medium / water mixture (70% / 30%) for 7h30 at 32 ° C. The propagation medium was then transferred to the fermentation medium at a rate of 2.5% / 97.5%. Fermentation was performed at 32 ° C. The initial pH of the propagation and fermentation media was adjusted to 5.0 without regulation. Urea has been added in propagation (1500 ppm) and in fermentation (1000 ppm). A dose of 0.06 mL / kg of commercial GA Spirizyme® Ultra Glucoamylase (Novozyme) solids was added in propagation but not in fermentation.
    The mass loss of the fermentation reactors was measured over time from t = 0 to t = 71 h.
    The mass loss results obtained during the alcoholic fermentation are shown in Figure 7.
    Figure 7 shows that the new strains provide both dextrin hydrolysis as fast as the 1-4998 strain and complete as the 1-4899 strain, but are also faster than the 1-4999 strain. . It can be concluded that the production of glucoamylase from Saccharomyces cerevisiae var. diastaticus has a stimulating effect on the hydrolytic activity of the glucoamylase Aspergillus niger. These strains do not only present a combination of fungal Aspergillus niger glucoamylase and Saccharomyces cerevisiae var. diastaticus (that is, with a kinetic profile between Aspergillus niger glucoamylase and Saccharomyces cerevisiae var. diastaticus glucoamylase), but have an improved kinetic profile with kinetic acceleration . There is thus a synergistic effect between the glucoamylase of fungal origin and that of Saccharomyces cerevisiae var. diastaticus
    The composition of the fermentation samples is measured by high performance liquid chromatography (HPLC) on an Aminex® HPX 87H column (Biorad) with a solution of 5 mM H2SO4 as eluent.
    The HPLCs carried out at the end of fermentation do not show any major defects for any of the strains considered (Table 4). They are a good reminder of the inability of the STA1 enzyme to completely hydrolyze dextrins unlike SFG and GLAA enzymes.
    Table 4: Concentrations after 71H fermentation (g / kg)
    权利要求:
    Claims (14)
    [1" id="c-fr-0001]
    1. A yeast strain of Saccharomyces cerevisiae, characterized in that it co-expresses: a gene encoding a glucoamylase of fungal origin; and a gene encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus.
    [2" id="c-fr-0002]
    2. Yeast strain of Saccharomyces cerevisiae according to claim 1, characterized in that the glucoamylase of Saccharomyces cerevisiae var. diastaticus has the protein sequence SEQ ID NO: 4.
    [3" id="c-fr-0003]
    A yeast strain of Saccharomyces cerevisiae according to claim 1 or 2, characterized in that the glucoamylase of fungal origin is selected from the group consisting of: Aspergillus niger glucoamylase, Saccharomycopsis fibuligera glucoamylase, Trichoderma glucoamylase reesei, a glucoamylase of Thermomyces lanuginosis, a glucoamylase of Rhizopus oryzae or a glucoamylase of Aspergillus oryzae,
    [4" id="c-fr-0004]
    4. Yeast strain of Saccharomyces cerevisiae according to claim 3, characterized in that the glucoamylase of fungal origin is a glucoamylase of Aspergillus niger or a glucoamylase of Saccharomycopsis fibuligera.
    [5" id="c-fr-0005]
    5. Yeast strain of Saccharomyces cerevisiae according to claim 4, characterized in that the glucoamylase of fungal origin is a glucoamylase of Aspergillus niger and has the protein sequence SEQ ID NO: 2.
    [6" id="c-fr-0006]
    6. A yeast strain of Saccharomyces cerevisiae according to any one of claims 1 to 5, characterized in that it comprises m copies of the gene encoding a fungal glucoamylase and n copies of the gene coding for the glucoamylase of Saccharomyces cerevisiae var. . diastaticus, wherein m is an integer from 2 to 10 and n is an integer from 2 to 10.
    [7" id="c-fr-0007]
    7. A yeast strain of Saccharomyces cerevisiae according to any one of claims 1 to 6, characterized in that the gene encoding a glucoamylase of fungal origin and that encoding the glucoamylase of Saccharomyces cerevisiae var. diastaticus are integrated within the genome of said yeast.
    [8" id="c-fr-0008]
    8. A yeast strain of Saccharomyces cerevisiae according to claim 1, said strain being the strain deposited on August 6, 2015 under the Budapest Treaty to the CNCM under the number I-5005.
    [9" id="c-fr-0009]
    9. A yeast strain of Saccharomyces cerevisiae according to claim 1, said strain being the strain deposited on July 9, 2015 under the Budapest Treaty to the CNCM under the number 1-4997.
    [10" id="c-fr-0010]
    10. Yeast strain of Saccharomyces cerevisiae characterized in that it contains the nucleic acid sequence SEQ ID NO: 1 and the nucleic sequence SEQ ID NO: 3.
    [11" id="c-fr-0011]
    11. A method for obtaining a yeast strain, said method comprising the following steps: a) genetic modification of a yeast of Saccharomyces cerevisiae so as to co-express a gene encoding a glucoamylase of fungal origin and a gene encoding glucoamylase & Saccharomyces cerevisiae var. diastaticus; b) culturing and fermentation of the strain obtained in step a) on a dextrin medium; c) selection of strains exhibiting fermentation kinetics at least equal to or greater than the strain deposited on 9 July 2015 under the Budapest Treaty to the CNCM under number 1-4999 under the same conditions.
    [12" id="c-fr-0012]
    12. A process for producing bioethanol from a biomass characterized in that it comprises the following steps: a) prehydrolysis and liquefaction of the starch of the biomass; b) contacting the liquefied starch obtained in step a) with a yeast as described in any one of claims 1 to 10; c) hydrolysis and fermentation of the liquefied starch by said yeast; d) extracting the ethanol produced in step c).
    [13" id="c-fr-0013]
    The method of claim 12, said method further comprising a step b ') of adding exogenous glucoamylase enzymes after step b) and / or during step c).
    [14" id="c-fr-0014]
    14. Use of a yeast strain according to any one of claims 1 to 10, for the production of bioethanol.
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    同族专利:
    公开号 | 公开日
    DK3344763T3|2021-11-22|
    BR112018004066A2|2018-12-11|
    EP3344763B1|2021-10-06|
    US20190292532A1|2019-09-26|
    CN108603186B|2022-01-11|
    WO2017037362A1|2017-03-09|
    FR3040395B1|2019-01-25|
    EP3344763A1|2018-07-11|
    PL3344763T3|2022-02-07|
    US10947519B2|2021-03-16|
    CN108603186A|2018-09-28|
    AR105862A1|2017-11-15|
    引用文献:
    公开号 | 申请日 | 公开日 | 申请人 | 专利标题
    WO2019063543A1|2017-09-29|2019-04-04|Dsm Ip Assets B.V.|Improved glycerol free ethanol production|
    CN111334446A|2018-12-19|2020-06-26|吉林中粮生化有限公司|High-temperature-resistant saccharifying yeast strain and application thereof|
    US11274310B2|2017-09-29|2022-03-15|Dsm Ip Assets B.V.|Yeast cells for glycerol free ethanol production|CN103038340A|2010-04-12|2013-04-10|斯泰伦博什大学|Biofuel production|FR3083245A1|2018-07-02|2020-01-03|Lesaffre Et Compagnie|SACCHAROMYCES CEREVISIAE STRAINS EXPRESSING EXOGENOUS GLUCOAMYLASE AND XYLANASE ENZYMES AND THEIR USE IN THE PRODUCTION OF BIOETHANOL|
    CN113052271B|2021-05-14|2022-02-15|江南大学|Biological fermentation data prediction method based on deep neural network|
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    优先权:
    申请号 | 申请日 | 专利标题
    FR1558079A|FR3040395B1|2015-08-31|2015-08-31|YEAST STRAINS CO-EXPRESSING EXOGENOUS GLUCOAMYLASES, PROCESS FOR OBTAINING THEM AND USE THEREOF FOR PRODUCING BIOETHANOL|
    FR1558079|2015-08-31|FR1558079A| FR3040395B1|2015-08-31|2015-08-31|YEAST STRAINS CO-EXPRESSING EXOGENOUS GLUCOAMYLASES, PROCESS FOR OBTAINING THEM AND USE THEREOF FOR PRODUCING BIOETHANOL|
    US15/755,675| US10947519B2|2015-08-31|2016-08-23|Yeast strains co-expressing exogenous glucoamylases, the method for obtaining said yeast strains and the use thereof to produce bioethanol|
    PL16770052T| PL3344763T3|2015-08-31|2016-08-23|Yeast strains co-expressing exogenous glucoamylases, the method for obtaining said yeast strains and the use thereof to produce bioethanol|
    DK16770052.5T| DK3344763T3|2015-08-31|2016-08-23|Yeast strains CO CO-EXPRESSING EXOGENE GLUCOAMYLASES, METHOD FOR OBTAINING ITS AND USING IT FOR BIOETHANOL PRODUCTION|
    BR112018004066A| BR112018004066A2|2015-08-31|2016-08-23|yeast strains that coexpress exogenous glucoamylases, a process for producing said yeast strains and their use to produce bioethanol|
    PCT/FR2016/052107| WO2017037362A1|2015-08-31|2016-08-23|Yeast strains co-expressing exogenous glucoamylases, the method for obtaining said yeast strains and the use thereof to produce bioethanol|
    CN201680056376.1A| CN108603186B|2015-08-31|2016-08-23|Yeast strain co-expressing exogenous saccharifying enzyme, method for obtaining yeast strain and application of yeast strain in production of bioethanol|
    EP16770052.5A| EP3344763B1|2015-08-31|2016-08-23|Yeast strains co-expressing exogenous glucoamylases, the method for obtaining said yeast strains and the use thereof to produce bioethanol|
    ARP160102643A| AR105862A1|2015-08-31|2016-08-30|LEAVES OF LEAVING COEXPRESSING EXOGEN GLUCOAMYLASES, PROCEDURE OF OBTAINING AND ITS USE TO PRODUCE BIOETHANOL|
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