标签归档:pcmv

pCMV-Myc载体说明书

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型号 载体名称 出品公司 载体用途 价格
VPC0050 pCMV-Myc Clontech 哺乳动物表达载体 800

 

产品参数: 

Key Function:Constitutive Expression
Promoter:CMV
Cloning Method:Restriction Enzyme/MCS
Constitutive or Inducible System:Constitutive

载体抗性: 

氨苄青霉素(Ampicillin)

载体描述: 

The pCMV-Myc Mammalian Expression Vector expresses proteins containing the N-terminal c-Myc epitope tag. The c-Myc epitope tag is well-characterized and highly immunoreactive. High-level expression in mammalian cells is driven from the human cytomegalovirus immediate early promoter/enhancer(P/CMVIE). The vector contains an intron(splice donor/splice acceptor); the epitope tag; an CMV IE MCS; and a polyadenylation signal from SV40. This vector also possesses the ampicillin resistance gene for selection in E.coli.

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pCMV-Tag 2B载体说明书

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型号 载体名称 出品公司 载体用途 价格
VPS0040 pCMV-Tag 2B Stratagene 哺乳动物表达载体 800

 

产品参数: 

Key Function:Constitutive Expression
Mammalian Selection:Neo,G418
Promoter:CMV
Cloning Method:Restriction Enzyme/MCS
Constitutive or Inducible System:Constitutive

载体抗性: 

卡那霉素(Kanamycin)

载体描述: 

Epitope tags provide a method to localize gene products in living cells, identify associated proteins, track the movement of tagged proteins within a cell, and characterize new genes without creating protein-specific antibodies. The pCMV-Tag1 vector contains both the synthetic FLAG epitopell ll and the c-myc epitope from the human c-myc gene. The pCMV-Tag1 vector allows production of fusion proteins in a variety of conformations. The pCMV-Tag2-5 vectors allow either c-myc or FLAG epitope tagging at either the C- or N-terminus. Each pCMV-Tag2-5 vector is supplied with all three reading frames for easy cloning and expression. The small size of the FLAG (eight amino acids long) and c-myc epitope tags (ten amino acids long) decreases the possibility of interference with the tagged protein. The FLAG and c-myc epitopes are recognized by the anti-c-myc and anti-FLAG antibodies, which can be used to characterize the target protein. The pCMV-Tag vectors allow high-level expression of tagged proteins in mammalian cells. Expression is driven by the human cytomegalovirus (CMV) immediate early promoter. The CMV promoter provides constitutive expression of cloned genes in a wide variety of cell lines. The translational start sequence used in the pCMV-Tag1, pCMV-Tag2 and pCMV-Tag3 vectors is a 10-base Kozak consensus sequence of CGG(A/G)CCATGG. pCMV-Tag4 and pCMV-Tag5 vectors do not contain a translation start sequence. Stable clone selection is made possible with G418 by the presence of the neomycin-resistance gene. The pCMV-Tag vectors are only 4.3 kb, allowing easy cloning and vector manipulations. This small size is due to the single antibiotic selection marker used by both prokaryotic and mammalian cells. The neomycin-resistance gene provides stable selection in mammalian cells with G418 driven by the SV40 promoter and kanamycin selection in E. coli cells driven by the bla (ß-lactamase) promoter.

 

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pCMV-Tag 5B载体说明书

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型号 载体名称 出品公司 载体用途 价格
VPS0545 pCMV-Tag 5B Stratagene 哺乳动物表达载体 800

 

产品参数: 

Key Function:Constitutive Expression
Mammalian Selection:Neo,G418
Promoter:CMV
Cloning Method:Restriction Enzyme/MCS
Constitutive or Inducible System:Constitutive

载体抗性: 

卡那霉素(Kanamycin)

载体描述: 

Epitope tags provide a method to localize gene products in living cells, identify associated proteins, track the movement of tagged proteins within a cell, and characterize new genes without creating protein-specific antibodies. The pCMV-Tag1 vector contains both the synthetic FLAG epitopell ll and the c-myc epitope from the human c-myc gene. The pCMV-Tag1 vector allows production of fusion proteins in a variety of conformations. The pCMV-Tag2-5 vectors allow either c-myc or FLAG epitope tagging at either the C- or N-terminus. Each pCMV-Tag2-5 vector is supplied with all three reading frames for easy cloning and expression. The small size of the FLAG (eight amino acids long) and c-myc epitope tags (ten amino acids long) decreases the possibility of interference with the tagged protein. The FLAG and c-myc epitopes are recognized by the anti-c-myc and anti-FLAG antibodies, which can be used to characterize the target protein. The pCMV-Tag vectors allow high-level expression of tagged proteins in mammalian cells. Expression is driven by the human cytomegalovirus (CMV) immediate early promoter. The CMV promoter provides constitutive expression of cloned genes in a wide variety of cell lines. The translational start sequence used in the pCMV-Tag1, pCMV-Tag2 and pCMV-Tag3 vectors is a 10-base Kozak consensus sequence of CGG(A/G)CCATGG. pCMV-Tag4 and pCMV-Tag5 vectors do not contain a translation start sequence. Stable clone selection is made possible with G418 by the presence of the neomycin-resistance gene. The pCMV-Tag vectors are only 4.3 kb, allowing easy cloning and vector manipulations. This small size is due to the single antibiotic selection marker used by both prokaryotic and mammalian cells. The neomycin-resistance gene provides stable selection in mammalian cells with G418 driven by the SV40 promoter and kanamycin selection in E. coli cells driven by the bla (ß-lactamase) promoter.

 

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pCMV-Tag 2A载体说明书

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型号 载体名称 出品公司 载体用途 价格
VPS0039 pCMV-Tag 2A Stratagene 哺乳动物表达载体 800

 

产品参数: 

Key Function:Constitutive Expression
Mammalian Selection:Neo,G418
Promoter:CMV
Cloning Method:Restriction Enzyme/MCS
Constitutive or Inducible System:Constitutive

载体抗性: 

卡那霉素(Kanamycin)

载体描述: 

Epitope tags provide a method to localize gene products in living cells, identify associated proteins, track the movement of tagged proteins within a cell, and characterize new genes without creating protein-specific antibodies. The pCMV-Tag1 vector contains both the synthetic FLAG epitopell ll and the c-myc epitope from the human c-myc gene. The pCMV-Tag1 vector allows production of fusion proteins in a variety of conformations. The pCMV-Tag2-5 vectors allow either c-myc or FLAG epitope tagging at either the C- or N-terminus. Each pCMV-Tag2-5 vector is supplied with all three reading frames for easy cloning and expression. The small size of the FLAG (eight amino acids long) and c-myc epitope tags (ten amino acids long) decreases the possibility of interference with the tagged protein. The FLAG and c-myc epitopes are recognized by the anti-c-myc and anti-FLAG antibodies, which can be used to characterize the target protein. The pCMV-Tag vectors allow high-level expression of tagged proteins in mammalian cells. Expression is driven by the human cytomegalovirus (CMV) immediate early promoter. The CMV promoter provides constitutive expression of cloned genes in a wide variety of cell lines. The translational start sequence used in the pCMV-Tag1, pCMV-Tag2 and pCMV-Tag3 vectors is a 10-base Kozak consensus sequence of CGG(A/G)CCATGG. pCMV-Tag4 and pCMV-Tag5 vectors do not contain a translation start sequence. Stable clone selection is made possible with G418 by the presence of the neomycin-resistance gene. The pCMV-Tag vectors are only 4.3 kb, allowing easy cloning and vector manipulations. This small size is due to the single antibiotic selection marker used by both prokaryotic and mammalian cells. The neomycin-resistance gene provides stable selection in mammalian cells with G418 driven by the SV40 promoter and kanamycin selection in E. coli cells driven by the bla (ß-lactamase) promoter.

 

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pCMV-VSV-G 载体序列

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 pCMV-VSV-G 载体序列

型号 载体名称 出品公司 载体用途
VMA0369 pCMV-VSV-G Addgene 慢病毒载体
产品参数: 

5′ sequencing primer: T7

载体抗性: 
氨苄青霉素(Ampicillin)
载体描述: 

Vector for constitutive expression of VSV-G glycoprotein. Also known as pHCMV-G or pHCMV-VSV-G.

Retroviruses are efficient tools for delivering heritable genes into the genome of dividing cells. pCMV-VSV-G expresses the G glycoprotein of the vesicular stomatitis virus (VSV-G) under the control of the CMV immediate-early promoter. VSV-G is used in pseudotyping of Moloney Murine Leukenia Virus(MMLV)-based retroviral vectors by mediating viral entry. VSV-G interacts with phospholipidcomponents of the target cell membrane and fosters the fusion of viral and cellular membranes. VSV-G does not require a cell surface receptor and can serve as a surrogate viral envelope protein. 
The vector contains the ampicillin-resistance gene for propagation and antibiotic selection in bacteria.

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pCMV-VSV-G载体序列

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 pCMV-VSV-G载体序列说明书

型号 载体名称 出品公司 载体用途
VMA0369 pCMV-VSV-G Addgene 慢病毒载体
产品参数: 

5′ sequencing primer: T7

载体抗性: 
氨苄青霉素(Ampicillin)
载体描述: 

Vector for constitutive expression of VSV-G glycoprotein. Also known as pHCMV-G or pHCMV-VSV-G.

Retroviruses are efficient tools for delivering heritable genes into the genome of dividing cells. pCMV-VSV-G expresses the G glycoprotein of the vesicular stomatitis virus (VSV-G) under the control of the CMV immediate-early promoter. VSV-G is used in pseudotyping of Moloney Murine Leukenia Virus(MMLV)-based retroviral vectors by mediating viral entry. VSV-G interacts with phospholipidcomponents of the target cell membrane and fosters the fusion of viral and cellular membranes. VSV-G does not require a cell surface receptor and can serve as a surrogate viral envelope protein. 
The vector contains the ampicillin-resistance gene for propagation and antibiotic selection in bacteria.

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pCMV-MCS

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pCMV-MCS

型号 载体名称 出品公司 载体用途
VXS0413 pCMV-MCS Stratagene 腺相关病毒系统

Molecule: pCMV-MCS, 4492 bps DNA Circular

File Name: .cm5, dated 09 Jul 2009

Description:

Notes: GenBank 4492 bp DNA circular

Molecule Features:

Start End Name Feature Key Draw As

9 667 CMV prom Gene

675 1167 Intron Gene

1175 1250 MCS Gene

1246 1732 pA Gene

1893 2560 Ori Gene

2708 3568 bla Gene

4087 4393 f1 Gene

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