We narrowed to 10,012 results for: SUB

pWS3808

• Plasmid: #185749
• Purpose: Sub-array spacer 4/4
• Depositor: Rodrigo Ledesma-Amaro
• Article: Shaw et al Nat Commun. 2022 Aug 25;13(1):4984. doi:
• Insert: CRISPRai sub-array spacer 4/4
• Use: CRISPR
• Available Since: Oct. 28, 2022
• Availability: Academic Institutions and Nonprofits only

pWS3807

• Plasmid: #185748
• Purpose: Sub-array spacer 3/4
• Depositor: Rodrigo Ledesma-Amaro
• Article: Shaw et al Nat Commun. 2022 Aug 25;13(1):4984. doi:
• Insert: CRISPRai sub-array spacer 3/4
• Use: CRISPR
• Available Since: Oct. 28, 2022
• Availability: Academic Institutions and Nonprofits only

Kohinoor 2.0/pcDNA3

• Plasmid: #182315
• Purpose: Positively reversibly photoswitchable fluorescent protein
• Depositor: Takeharu Nagai
• Article: Wazawa et al Microscopy (Oxf). 2021 Aug 9;70(4):340-3
• Insert: Kohinoor 2.0
• Tags: No tag
• Expression: Mammalian
• Promoter: T7 promoter
• Available Since: May 16, 2022
• Availability: Academic Institutions and Nonprofits only

pLenti-CMV-Pink Flamindo-p2a-paGFP-bPAC-CAAX

• Plasmid: #202718
• Purpose: Mammalian co-expression of soluble Pink Flamindo and membrane-bound bPAC for cAMP perturbation and imaging
• Depositor: Adam Cohen
• Article: Xiang et al bioRxiv 2023
• Inserts: Pink Flamindo; paGFP-bPAC-CAAX
• Use: Lentiviral
• Expression: Mammalian
• Promoter: CMV
• Available Since: Aug. 3, 2023
• Availability: Academic Institutions and Nonprofits only

pSU19mCherry

• Plasmid: #225181
• Purpose: Medium copy cloning vector with mCherry integrated in the multiple cloning site. There is a SmaI immediately upstream of mCherry start codon, which allows for C-terminal mCherry fusions.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: mCherry
• Expression: Bacterial
• Available Since: Nov. 14, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT031

• Plasmid: #225177
• Purpose: Low copy cloning vector with mCherry integrated in the multiple cloning site (AmpR). There is a SmaI immediately upstream of mCherry start codon, which allows for C-terminal mCherry fusions.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: mCherry
• Expression: Bacterial
• Available Since: Sept. 23, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT034

• Plasmid: #225180
• Purpose: Low copy cloning vector with mCherry integrated in the multiple cloning site (SmR). There is a SmaI immediately upstream of mCherry start codon, which allows for C-terminal mCherry fusions.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: mCherry
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT032

• Plasmid: #225178
• Purpose: Low copy cloning vector with mCherry integrated in the multiple cloning site (TetR). There is a SmaI immediately upstream of mCherry start codon, which allows for C-terminal mCherry fusions.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: mCherry
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT033

• Plasmid: #225179
• Purpose: Low copy cloning vector with mCherry integrated in the multiple cloning site (GmR). There is a SmaI immediately upstream of mCherry start codon, which allows for C-terminal mCherry fusions.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: mCherry
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT030

• Plasmid: #225176
• Purpose: Low copy cloning vector with mCherry integrated in the multiple cloning site (Chlr). There is a SmaI immediately upstream of mCherry start codon, which allows for C-terminal mCherry fusions.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: mCherry
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pLenti-CMV-Myr-Pink Flamindo-p2a-EGFP-bPAC

• Plasmid: #202717
• Purpose: Mammalian co-expression of membrane-bound Pink Flamindo and soluble bPAC for cAMP perturbation and imaging
• Depositor: Adam Cohen
• Article: Xiang et al bioRxiv 2023
• Inserts: Myr-Pink Flamindo; EGFP-bPAC
• Use: Lentiviral
• Tags: 10xHis and myc
• Expression: Mammalian
• Promoter: CMV
• Available Since: Aug. 3, 2023
• Availability: Academic Institutions and Nonprofits only

pHBJT001

• Plasmid: #225152
• Purpose: High copy cloning vector for integration of C-terminal FLAG epitope tag. SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in same orientation as lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 9, 2024
• Availability: Academic Institutions and Nonprofits only

pLenti-CMV-Myr-Pink Flamindo-p2a-EGFP-bPAC-CAAX

• Plasmid: #202719
• Purpose: Mammalian co-expression of membrane-bound Pink Flamindo and membrane-bound bPAC for cAMP perturbation and imaging
• Depositor: Adam Cohen
• Article: Xiang et al bioRxiv 2023
• Inserts: Myr-Pink Flamindo; EGFP-bPAC-CAAX
• Use: Lentiviral
• Expression: Mammalian
• Promoter: CMV
• Available Since: Aug. 3, 2023
• Availability: Academic Institutions and Nonprofits only

pHBJT011

• Plasmid: #225162
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (GmR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in same orientation as lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 25, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT008

• Plasmid: #225159
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (AmpR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in opposite orientation of lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 23, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT007

• Plasmid: #225158
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (AmpR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in same orientation as lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 23, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT014

• Plasmid: #225165
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (SmR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in opposite orientation of lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT013

• Plasmid: #225164
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (SmR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in same orientation as lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT012

• Plasmid: #225163
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (GmR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in opposite orientation of lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only

pHBJT010

• Plasmid: #225161
• Purpose: Low copy cloning vector for integration of C-terminal FLAG epitope tag (TetR). SmaI restriction site immediately upstream of the FLAG epitope. FLAG epitope in opposite orientation of lac promoter.
• Depositor: Jenny-Lee Thomassin
• Article: Braun et al J Biosci Bioeng. 2024 Sep 6:S1389-1723(2
• Type: Empty backbone
• Use: Synthetic Biology
• Tags: FLAG epitope tag (35 bp)
• Expression: Bacterial
• Available Since: Sept. 10, 2024
• Availability: Academic Institutions and Nonprofits only