Cadherins are calcium-dependent cell adhesion proteins that preferentially interact with themselves in a homophilic manner in connecting cells. Cadherins thus contribute to the sorting of heterogeneous cell types. CDHR5 (Cadherin-related family member 5) is an 845 amino acid (aa) single pass type I transmembrane protein of the cadherin superfamily. CDHR5 contains an N-terminal signal peptide, a 644-aa extracellular domain (ECD) with 4 cadherin domains, 4 31-aa tandem repeats and 8 potential glycosylation sites, a transmembrane domain (TM), and a 155-aa cytoplasmic tail. CDHR1 is a novel mucin-like member of the cadherin superfamily. In addtion to cadherin domains, CDHR5 also contains nonpolymorphic tandem repeats rich in proline, serine and threonine similar to mucin proteins. The role of the hybrid extracellular region and the specific function of CDHR5 have not yet been determined.
Gene Symbol: CDHR5; MLPCDH; MUCDHL; MUPCDH; MU-PCDH
NCBI Gene ID: 53841
Uniprot Entry: Q9HBB8
Construct Details: Full length human CDHR5 gene is subcloned into the Lentiviral expression vector pLTC with an upstream CMV promoter and with or without a selection marker, which can be used for both transient and stable expression in mammalian cells. It can be co-transfected with the LentiPAK DNA mix (SKU# LP-001) into HEK293 cells to produce high titer lentiviral particles. Multiple choices of a stable antibiotic selection marker are available.
Vector Type: pLTC or pLTC-IRES-Marker (lentiviral expression vector containing a heterologous CMV promoter +/- a selection marker, see the vector map above)
Gene Insert Size: 2538 (bp)
Gene Insert Sequence:
ATGGGGTCTTGGGCCCTGCTGTGGCCTCCCCTGCTGTTCACCGGGCTGCTCGTCCGACCCCCGGGGACCA
TGGCCCAGGCCCAGTACTGCTCTGTGAACAAGGACATCTTTGAAGTAGAGGAGAACACAAATGTCACCGA
GCCGCTGGTGGACATCCACGTCCCGGAGGGCCAGGAGGTGACCCTCGGAGCCTTGTCCACCCCCTTTGCA
TTTCGGATCCAGGGAAACCAGCTGTTTCTCAACGTGACTCCTGATTACGAGGAGAAGTCACTGCTTGAGG
CTCAGCTGCTGTGTCAGAGCGGAGGCACATTGGTGACCCAGCTAAGGGTGTTCGTGTCAGTGCTGGACGT
CAATGACAATGCCCCCGAATTCCCCTTTAAGACCAAGGAGATAAGGGTGGAGGAGGACACGAAAGTGAAC
TCCACCGTCATCCCCGAGACGCAACTGCAGGCTGAGGACCGCGACAAGGACGACATTCTGTTCTACACCC
TCCAGGAAATGACAGCAGGTGCCAGTGACTACTTCTCCCTGGTGAGTGTAAACCGTCCCGCCCTGAGGCT
GGACCGGCCCCTGGACTTCTACGAGCGGCCGAACATGACCTTCTGGCTGCTGGTGCGGGACACTCCGGGG
GAGAATGTGGAACCCAGCCACACTGCCACCGCCACACTAGTGCTGAACGTGGTGCCCGCCGACCTGCGGC
CCCCGTGGTTCCTGCCCTGCACCTTCTCAGATGGCTACGTCTGCATTCAAGCTCAGTACCACGGGGCTGT
CCCCACGGGGCACATACTGCCATCTCCCCTCGTCCTGCGTCCCGGACCCATCTACGCTGAGGACGGAGAC
CGCGGCATCAACCAGCCCATCATCTACAGCATCTTTAGGGGAAACGTGAATGGTACATTCATCATCCACC
CAGACTCGGGCAACCTCACCGTGGCCAGGAGTGTCCCCAGCCCCATGACCTTCCTTCTGCTGGTGAAGGG
CCAACAGGCCGACCTTGCCCGCTACTCAGTGACCCAGGTCACCGTGGAGGCTGTGGCTGCGGCCGGGAGC
CCGCCCCGCTTCCCCCAGAGACTGTATCGTGGCACCGTGGCGCGTGGCGCTGGAGCGGGCGTTGTGGTCA
AGGATGCAGCTGCCCCTTCTCAGCCTCTGAGGATCCAGGCTCAGGACCCGGAGTTCTCGGACCTCAACTC
GGCCATCACATATCGAATTACCAACCACTCACACTTCCGGATGGAGGGAGAGGTTGTGCTGACCACCACC
ACACTGGCACAGGCGGGAGCCTTCTACGCAGAGGTTGAGGCCCACAACACGGTGACCTCTGGCACCGCAA
CCACAGTCATTGAGATACAAGTTTCCGAACAGGAGCCCCCCTCCACAGATGTCCCCCCATCCCCAGAGGC
TGGAGGAACAACTGGGCCCTGGACCAGCACCACTTCCGAGGTCCCCAGACCCCCTGAGCCCTCCCAGGGA
CCCTCCACGACCAGCTCTGGGGGAGGCACAGGCCCTCATCCACCCTCTGGCACAACTCTGAGGCCACCAA
CCTCGTCCACACCCGGGGGGCCCCCGGGTGCAGAAAACAGCACCTCCCACCAACCAGCCACTCCCGGTGG
GGACACAGCACAGACCCCAAAGCCAGGAACCTCTCAGCCGATGCCCCCCGGTGTGGGAACCAGCACCTCC
CACCAACCAGCCACACCCAGTGGGGGCACAGCACAGACCCCAGAGCCAGGAACCTCTCAGCCGATGCCCC
CCAGTATGGGAACCAGCACCTCCCACCAACCAGCCACACCCGGTGGGGGCACAGCACAGACCCCAGAGGC
AGGAACCTCTCAGCCGATGCCCCCCGGTATGGGAACCAGCACCTCCCACCAACCAACCACACCCGGTGGG
GGCACAGCACAGACCCCAGAGCCAGGAACCTCTCAGCCGATGCCCCTCAGCAAGAGCACCCCATCTTCAG
GTGGCGGCCCCTCGGAGGACAAGCGCTTCTCGGTGGTGGATATGGCGGCCCTGGGCGGGGTGCTGGGTGC
GCTGCTGCTGCTGGCTCTCCTTGGCCTCGCCGTCCTTGTCCACAAGCACTATGGCCCCCGGCTCAAGTGC
TGCTGTGGCAAAGCTCCGGAGCCCCAGCCCCAAGGCTTTGACAACCAGGCGTTCCTCCCTGACCACAAGG
CCAACTGGGCGCCCGTCCCCAGCCCCACGCACGACCCCAAGCCCGCGGAGGCACCGATGCCCGCAGAGCC
CGCACCCCCCGGCCCTGCCTCCCCAGGCGGTGCCCCTGAGCCCCCCGCAGCGGCCCGAGCTGGCGGAAGC
CCCACGGCGGTGAGGTCCATCCTGACCAAGGAGCGGCGGCCGGAGGGCGGGTACAAGGCTGTCTGGTTTG
GCGAGGACATCGGGACGGAGGCAGACGTGGTCGTTCTCAACGCGCCCACCCTGGACGTGGATGGCGCCAG
TGACTCCGGCAGCGGCGATGAGGGCGAGGGCGCGGGGAGGGGTGGGGGTCCCTACGATGCGCCCGGTGGT
GATGACTCCTACATCTAA
Formulation: pre-packaged viral particles in the conditional medium (serum-free) from HEK293 cells (typical titer 106 - 107 IFU/ml)
FOR RESEARCH USE ONLY. NOT FOR DIAGNOSTIC OR THERAPEUTIC USE IN HUMAN.
Important Safety Information: With the safety features in place, our lentiviral vectors and viral particles can be employed in standard Biosafety Level 2 tissue culture facilities and should be treated with the same level of caution as any other potentially infectious agent. Any investigator who purchases our lentiviral/retroviral products & services is responsible for following Biosafety Level 2 requirements on the handling of viral particles. For more information on Biosafety Level 2 agents and practices, please refer to NIH’s “Biosafety Considerations for Research with Lentiviral Vectors”.
Restriction: This product is not transferable or re-sellable. Customer obtain no right to transfer, assign, or sublicense its use rights, or to transfer, resell, package, or otherwise distribute the product, or to use the product for the benefit of any third party or for any commercial purpose. Customer may only use the product in compliance with applicable local, state and federal laws, regulations and rules. Customer may not directly or indirectly use the product or allow the transfer, transmission, export or re-export of all or any part of the product in violation of any export control law or regulation of the united states or any other relevant jurisdiction. Your use of this product constitutes acceptance of the terms of this limited use agreement. Please refer to our “terms & conditions” for details. If you are not willing to accept the limitation of this agreement, G&P Biosciences will accept return of the product for a full/partial refund.
Pre-packaged lentiviral particles are most advanced gene delivery tools. Each particles contain a fully sequence verified target gene and are psudotyped with the VSV-G glycoprotein, ready for transduction into into a wide range of cell types including hard-to-transfect primary cells and non-dividing cells. They are supplied in 1-mL aliquot(s) of the serum-/antibiotic-free solution suitable for both in vitro and in vivo delivery. They are produced in HEK293 packaging cells with a typical titer of ≥107 IFU/ml using our optimized LentPAKTM packaging system. The lentiviral particles can be used to transduce subconfluent target cells. Depending on your purpose, you may choose a specific multiplicity of infection (MOI) or test a range of MOIs to determine which gives you the desired results. Transduction can be enhanced by the addition of polybrene, also known as hexadimethrine bromide (typically at 8-10 μg/ml).
Quick Protocol for Transduction
Day 1. Seeding Target Cells
For an example, plate target cells in a 10 cm plate at a density of 1 - 5x 105 cells/ml that will produce approximately 60% confluency in 24 hours.
Note: other size plates can also be used depending on the nature of your experiment. Adjust the reagent amount according to Table 1
Table 1. Seeding Density of Target Cells (1 day prior to transduction)
Vessel Type |
Seeding Target Cell# |
Volume of Media |
10-cm dish |
1 – 5 x 106 |
10 mL |
6-well plate |
0.3 – 1 x 106 |
2 mL/well |
12-well plate |
0.15 – 0.5 x 106 |
1 mL/well |
24-well plate |
0.6 – 2 x 105 |
0.5 mL/well |
96-well plate |
1 – 4 x 104 |
0.1 mL/well |
Day 2. Transduction
Remove the growth media from the dish/plate prepared the day before. Replace with 1/2 volume of culture medium containing desired amount of lentiviral particles (at 2 to 20 MOI). For example, add 4.5 mL of growth medium and 0.5 mL of Lentiviral particles, or simply add 5 mL of Lentiviral particles (for a low titer viral preparation or a high MOI transduction). Add polybrene directly to the media on the target cells at 8 μg/ml. Mix by gentle swirling.
Incubate at 37°C with 5% CO2 for 4 - 24 hours, then replace the transduction medium with right amount of growth medium according to table 1 (for example 10 mL for 10-cm dish). Culture the cells for 48 – 72 hours, and transduced cells are ready for downstream analyses.
Note: Adjust volumes accordingly for transduction of other plate types. For example, add 1 ml of growth medium and lentiviral particle mixture for 6-well plate, 0.5 ml for 12-well and 0.25 mL for 24-well except for 96 well, in which 100 μl should be used. The change of transduction medium is often unnecessary with our pre-packaged lentiviral particles. Simply culture cells for 3-4 days before analysis.
The virus-containing media can be changed in as short as 4 hours after transduction if toxicity of the lentiviral transduction is a concern. Normally reverse transcription and genome integration of the lentivector takes place within 24-36 hours. With our ready-to-use, prepackaged lentiviral particles, the change of media is often unnecessary. The transduction process can be ongoing for 2 - 6 days without significant impact on cell growth/viability. The transduction process can also be repeated if desired. For a lentivector with a fluorescent reporter (such as GFP), FACS can be used to enrich for cells that express GFP. If it contains a drug selectable marker, follow the protocol for the particular drug. For example, puromycin selection is usually carried out at 1-10 μg/mL, depending on the target cells’ sensitivity
Important Safety Information
With the safety features in place, our lentiviral vectors and viral particles can be employed in standard Biosafety Level 2 tissue culture facilities and should be treated with the same level of caution as any other potentially infectious agent. Any investigator who purchases our lentiviral/retroviral products & services is responsible for following Biosafety Level 2 requirements on the handling of viral particles. For more information on Biosafety Level 2 agents and practices, please refer to NIH’s “Biosafety Considerations for Research with Lentiviral Vectors”.
Poor Transduction Efficiency:
Poor transduction efficiency could be due to a low viral titer. While lentivectors can accommodate relatively large inserts (up to 8 kb) comparing to other systems, there is still a packaging limit. In general, lentivectors could transfer up to 8-kb gene inserts. However, any gene insert larger than 4kb will dramatically decreases packaging efficiency, which would results in a lower viral titer. To overcome low titers, concentrate viral particles or lower target cell density for transduction. If the transduction efficiency is low despite a high titer of virus, the total volume of transduction media on the target cells may be too high. Transduction can be carried out in a volume of media that just covers the cells; this may increase the exposure of the cells to the virus. Low speed spin (e.g., 1500 rpm for 15-30 min) may help increase the likelihood of virus-cell interactions. Pseudotyping of the transducing virus to target more abundant receptors on a particular cell type is another potential approach.
Transduction Kills Target Cells:
It is possible that MOI may be too high. Perform the transduction with a lower MOI or less viral particles. Packaging cell medium may not be compatible for target cell growth. Either dilute the virus in target cell-compatible medium or concentrate and resuspend the virus in medium compatible with the target cell growth. Change the transduction media containing the virus as early as 4 hrs after transduction.
FOR RESEARCH USE ONLY. NOT FOR DIAGNOSTIC OR THERAPEUTIC USE IN HUMAN.
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