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sucrose counter selectable pre112 (Addgene inc)

Name: sucrose counter selectable pre112
Brand: Addgene inc
Rating: 93 (16 reviews)

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Addgene inc sucrose counter selectable pre112

Fig. 1 Schematic map of suicide vectors. A All suicide vectors were derived from pHY093 <t>(pRE112-Cm-GFP)</t> or pHY094 (pRE112-Kan-GFP). B Two homologous arms, i.e., HA_up and HA_down were cloned from E. coli W3110 genome and fused together by fusion PCR. The fused homologous arms replaced the GFP cassette in pHY093 (pRE112-Cm-GFP), resulting in pHY095 (pRE112-Cm-ΔOAg). C the viaB_locus was cloned from S. Typhi genome. The linearized pHY095 (pRE112-Cm-ΔOAg) vector and viaB_locus were assembled in vitro, resulting in pHY129 (pRE112-Cm-ΔOAg::viaB locus). D A cassette of FRT-flanked chloramphenicol resistance gene was cloned from pCP3, and cloned into the middle of homologous arms, resulting in pHY099 (pRE112-Km-ΔOAg::Cm_FRT2). E The OAgST O-antigen gene cluster was cloned from S. Typhimurium genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgST were assembly in vitro, resulting in pHY100 (pRE112-Km-ΔOAg::OAgST-Cm_FRT2). F The OAgSE O-antigen gene cluster was cloned from S. Enteritidis genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgSE were assembly in vitro, resulting in pHY101 (pRE112-Km-ΔOAg::OAgSE-Cm_FRT2). G pHY102 (pRE112-Km-ΔOAg::OAgSA-Cm_FRT2) was derived from pHY101 by deliberately deleting the tyv gene

Sucrose Counter Selectable Pre112, supplied by Addgene inc, used in various techniques. Bioz Stars score: 93/100, based on 16 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/sucrose counter selectable pre112/product/Addgene inc
Average 93 stars, based on 16 article reviews

sucrose counter selectable pre112 - by Bioz Stars, 2026-02

93/100 stars

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1) Product Images from "Genetic engineering of E. coli K-12 for heterologous carbohydrate antigen production."

Article Title: Genetic engineering of E. coli K-12 for heterologous carbohydrate antigen production.

Journal: Microbial cell factories

doi: 10.1186/s12934-025-02749-2

Fig. 1 Schematic map of suicide vectors. A All suicide vectors were derived from pHY093 (pRE112-Cm-GFP) or pHY094 (pRE112-Kan-GFP). B Two homologous arms, i.e., HA_up and HA_down were cloned from E. coli W3110 genome and fused together by fusion PCR. The fused homologous arms replaced the GFP cassette in pHY093 (pRE112-Cm-GFP), resulting in pHY095 (pRE112-Cm-ΔOAg). C the viaB_locus was cloned from S. Typhi genome. The linearized pHY095 (pRE112-Cm-ΔOAg) vector and viaB_locus were assembled in vitro, resulting in pHY129 (pRE112-Cm-ΔOAg::viaB locus). D A cassette of FRT-flanked chloramphenicol resistance gene was cloned from pCP3, and cloned into the middle of homologous arms, resulting in pHY099 (pRE112-Km-ΔOAg::Cm_FRT2). E The OAgST O-antigen gene cluster was cloned from S. Typhimurium genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgST were assembly in vitro, resulting in pHY100 (pRE112-Km-ΔOAg::OAgST-Cm_FRT2). F The OAgSE O-antigen gene cluster was cloned from S. Enteritidis genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgSE were assembly in vitro, resulting in pHY101 (pRE112-Km-ΔOAg::OAgSE-Cm_FRT2). G pHY102 (pRE112-Km-ΔOAg::OAgSA-Cm_FRT2) was derived from pHY101 by deliberately deleting the tyv gene

Figure Legend Snippet: Fig. 1 Schematic map of suicide vectors. A All suicide vectors were derived from pHY093 (pRE112-Cm-GFP) or pHY094 (pRE112-Kan-GFP). B Two homologous arms, i.e., HA_up and HA_down were cloned from E. coli W3110 genome and fused together by fusion PCR. The fused homologous arms replaced the GFP cassette in pHY093 (pRE112-Cm-GFP), resulting in pHY095 (pRE112-Cm-ΔOAg). C the viaB_locus was cloned from S. Typhi genome. The linearized pHY095 (pRE112-Cm-ΔOAg) vector and viaB_locus were assembled in vitro, resulting in pHY129 (pRE112-Cm-ΔOAg::viaB locus). D A cassette of FRT-flanked chloramphenicol resistance gene was cloned from pCP3, and cloned into the middle of homologous arms, resulting in pHY099 (pRE112-Km-ΔOAg::Cm_FRT2). E The OAgST O-antigen gene cluster was cloned from S. Typhimurium genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgST were assembly in vitro, resulting in pHY100 (pRE112-Km-ΔOAg::OAgST-Cm_FRT2). F The OAgSE O-antigen gene cluster was cloned from S. Enteritidis genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgSE were assembly in vitro, resulting in pHY101 (pRE112-Km-ΔOAg::OAgSE-Cm_FRT2). G pHY102 (pRE112-Km-ΔOAg::OAgSA-Cm_FRT2) was derived from pHY101 by deliberately deleting the tyv gene

Techniques Used: Derivative Assay, Clone Assay, Plasmid Preparation, In Vitro, Long Range PCR

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Image Search Results

Journal: Microbial cell factories

Article Title: Genetic engineering of E. coli K-12 for heterologous carbohydrate antigen production.

doi: 10.1186/s12934-025-02749-2

Figure Lengend Snippet: Fig. 1 Schematic map of suicide vectors. A All suicide vectors were derived from pHY093 (pRE112-Cm-GFP) or pHY094 (pRE112-Kan-GFP). B Two homologous arms, i.e., HA_up and HA_down were cloned from E. coli W3110 genome and fused together by fusion PCR. The fused homologous arms replaced the GFP cassette in pHY093 (pRE112-Cm-GFP), resulting in pHY095 (pRE112-Cm-ΔOAg). C the viaB_locus was cloned from S. Typhi genome. The linearized pHY095 (pRE112-Cm-ΔOAg) vector and viaB_locus were assembled in vitro, resulting in pHY129 (pRE112-Cm-ΔOAg::viaB locus). D A cassette of FRT-flanked chloramphenicol resistance gene was cloned from pCP3, and cloned into the middle of homologous arms, resulting in pHY099 (pRE112-Km-ΔOAg::Cm_FRT2). E The OAgST O-antigen gene cluster was cloned from S. Typhimurium genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgST were assembly in vitro, resulting in pHY100 (pRE112-Km-ΔOAg::OAgST-Cm_FRT2). F The OAgSE O-antigen gene cluster was cloned from S. Enteritidis genome via Long-range PCR. The linearized pHY099 (pRE112-Km-ΔOAg::Cm_FRT2) vector and OAgSE were assembly in vitro, resulting in pHY101 (pRE112-Km-ΔOAg::OAgSE-Cm_FRT2). G pHY102 (pRE112-Km-ΔOAg::OAgSA-Cm_FRT2) was derived from pHY101 by deliberately deleting the tyv gene

Article Snippet: The gene cluster insertion mutations on the E. coli chromosome were constructed using the sucrose counter-selectable pRE112 (addgene, plasmid #43,828) suicide vectors [24].

Techniques: Derivative Assay, Clone Assay, Plasmid Preparation, In Vitro, Long Range PCR