Method for preparing cordyceps militaris polysaccharide through multi-gene combined expression
A technology of Cordyceps militaris polysaccharides and Cordyceps militaris, which is applied in the fields of genetic engineering and food and medicine, and can solve problems such as no inhibition of Escherichia coli and filamentous fungi, inability to meet the demand for polysaccharide products, and low polysaccharide production
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Embodiment 1
[0031] Embodiment 1 constructs the Cordyceps militaris strain that expresses pgm and ugdh in combination
[0032] Table 1 Sources of materials
[0033]
[0034] Table 2 Each medium component
[0035]
[0036]
[0037] The composition of the LB liquid medium: tryptone 10g / L, yeast extract 5g / L, NaCl 10g / L, solvent is distilled water, pH7.0.
[0038] The composition of the LB solid medium: tryptone 10g / L, yeast extract 5g / L, NaCl 10g / L, agar 15-20g / L, solvent is distilled water, pH 7.0.
[0039] The composition of the IM medium: 0.145% KH 2 PO 4 , 0.205%K 2 HPO 4 , 0.06% MgSO 4 ·7H 2 O, 0.03% NaCl, 0.01‰CaCl 2 , 0.001‰FeSO 4 , 0.05% NH 4 NO 3 , 5mL / L glycerin, 0.2% glucose, 5mL / L trace element stock solution, 40mL / L MES buffer solution (1mol / L, pH=5.5), solvent is distilled water; Described every 10ml trace element stock solution composition: ZnSO 4 ·7H 2 O 0.001g, CuSO 4 ·5H 2 O 0.001g, H 3 BO 4 0.001g, (NH 4 ) 2 SO 4 0.5g, MnSO 4 ·H 2 O0.001g, ...
Embodiment 2
[0066] Embodiment 2 constructs the Cordyceps militaris strain that expresses ugp and ugdh in combination
[0067] With the method of Example 1, the recombinant vector pCAMBIA-PgpdA-ugp-Tcbh1-hph-PtrpC was amplified by PCR using primers Insert-CobF&Insert-CobFR to obtain the insert fragment PgpdA-ugp-Tcbh1; using primers Plasmid-CobF&Plasmid-CobR to amplify the recombinant vector pCAMBIA -PgpdA-ugdh-Tcbh1-hph-PtrpC linearization.
[0068] use Seamless Cloning and Assembly Kit connects the insert to the linearized vector to obtain the combined expression recombinant vector PCAMBIA-PgpdA-ugp-ugdh-Tcbh1-hph-PtrpC (referred to as ugp-ugdh), such as figure 2 .
[0069] Other operations are the same as in Example 1, to obtain a genetically engineered strain of Cordyceps militaris expressing ugp and ugdh, and use forward primer F: 5'-CTATTCCTTTGCCCTCGGACGA-3' and reverse primer R: 5'-ATGCCTGAACTCACCGCGACGT-3' for PCR verification , to check whether the conversion is successful, t...
Embodiment 3
[0070] Embodiment 3 constructs the Cordyceps militaris bacterial strain that expresses pgm and ugp in combination
[0071] With the method of Example 1, the recombinant vector pCAMBIA-PgpdA-ugp-Tcbh1-hph-PtrpC was amplified by PCR using primers Insert-CobF&Insert-CobR to obtain the insert fragment PgpdA-ugp-Tcbh1; using primers Plasmid-CobF&Plasmid-CobR to amplify the recombinant vector pCAMBIA -PgpdA-pgm-Tcbh1-hph-PtrpC linearization.
[0072] use The Seamless Cloning and Assembly Kit connects the insert to the linearized vector to obtain the combined expression recombinant vector PCAMBIA-PgpdA-pgm-ugp-Tcbh1-hph-PtrpC (referred to as pgm-ugp), such as figure 2 .
[0073] Other operations are the same as in Example 1, obtain the Cordyceps militaris genetically engineered bacterial strain that expresses pgm and ugp in combination, and carry out PCR verification with forward primer F: 5'-CTATTCCTTTGCCCTCGGACGA-3' and reverse primer R: 5'-ATGCCTGAACTCACCGCGACGT-3' , to check ...
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