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  1. Pouring LB Agar Plates

    Type
    Protocol
    ... Protocols Pouring LB Agar Plates Pouring LB Agar Plates You may also like......solidifies in the bottle while you’re pouring, you should stop pouring and re-make the gel-mix. If you’re... autoclave tape. The autoclave tape will darken during the autoclave process if your sample has spent ...in the autoclave, you should prepare your plate pouring station: Find an empty section of lab bench with... the flame just to the side of where you’ll be pouring your plates - be sure to leave room for your bottle...appropriate antibiotics, and a section for active pouring. Prepare your antibiotics. Prior to adding your...1000x stock solution. For example: If you’ll be preparing plates with a final concentration of 100 ug/mL...

  2. Fluorescence Titering Assay

    Type
    Protocol
    ... Protocols Fluorescence Titering Assay Fluorescence Titering Assay for Lentivirus You may also...cells and debris. Lentiviral titer can decrease during cycles of freeze-thaw. If you are freezing and ...consider wells with less than 40% fluorescent cells. Titering methods assume one integration event per cell....

  3. Colony Formation Titering Assay

    Type
    Protocol
    ... Protocols Colony Formation Titering Assay Colony Formation Titering Assay for Lentivirus You may also...luer-lock filter, Corning 431229 10 mL luer-lock syringe, BD BD300912 0.45 μm polyethersulfone filter, Nalgene...added at the time of viral transduction, and not during the cell seeding step. Procedure Before beginning...cells and debris. Lentiviral titer can decrease during cycles of freeze-thaw. If you are freezing and ...

  4. Handling Plasmids from Addgene - Purifying Plasmid DNA

    Type
    Protocol
    ... Protocols Recovering Plasmid DNA from Bacterial Culture Recovering Plasmid DNA from Bacterial...with your plasmid Resuspension buffer Denaturing solution Renaturing solution 2 mg/mL RNase A TE or water-saturated...solution. Add a renaturing solution to the denatured bacteria. Note: This step brings the pH back down...that is compatible with the next solution. Add a denaturing solution to the resuspended bacteria. Note: This...mM EDTA Store Solution I at 4°C Solution II - Denaturing Solution 0.2 N NaOH 1.0% SDS Store Solution II... II at room temperature Solution III - Renaturing Solution (Potassium Acetate) 120 mL 5M Potassium acetate...supernatant into a new tube by pipetting or carefully pouring. Optional: Add 5 μL of 2 mg/mL RNase A to the supernatant...

  5. Transfection for Recombinant Antibodies

    Type
    Protocol
    ...a variety of applications. Sharing speeds science. We believe that sharing the full details of our protocols...mL luer-lock syringe, BD BD302832 0.2 µm luer-lock filter, VWR 431229 0.22 µm PES filtering system, 1000...1000 mL, VWR 431098 0.45 µm PES filtering system, 500 mL, VWR 430770 Trypan Blue, Thermo Fisher T10282 ... reagents Store at 4 °C until use. We suggest preparing fresh solutions after one month. BCD Feed 500 ... Glutagro Store at 4 °C until use. We suggest preparing fresh solutions after one month. 1000X protease...mL) Mix well and sterilize through a 0.2 µm PES syringe filter. Aliquot and freeze upright at -20 °C. Procedure...Section 3: BCD Feed and valproic acid supplementation During the 24–144 h post-transfection, supplement the ...

  6. Kit Free RNA Extraction

    Type
    Protocol
    ...to a refrigerated centrifuge, you can carefully bring a centrifuge into a cold room for centrifugation...centrifugation. Once you’re done using the centrifuge, bring this equipment back to room temperature, as prolonged...Add the correct amount of 7.5 M LiCl solution to bring the concentration of LiCl in the extracted aqueous...sample, consider making smaller aliquots of it and storing those in -80°C. Option #2 - TRIzol® Protocol Homogenize...

  7. Protocol - pLKO.1 – TRC Cloning Vector

    Type
    Protocol
    ...siRNA selection tool to determine a set of top-scoring targets for your gene. For example, the Whitehead...alleviate concerns about off-target effects. B.2 Ordering Oligos Compatible with pLKO.1 To generate oligos... 5 μL 10x NEB buffer 1 1 μL AgeI add ddH 2 O to bring to 50 μL final volume Incubate at 37°C for 2 hours...ligase buffer 1 μL NEB T4 DNA ligase add ddH 2 O to bring to 20 μL final volume Incubate at 16°C for 4-20 ...for EcoRI 0.8 μL EcoRI 0.8 μL NcoI add ddH 2 O to bring to 20 μL final volume Incubate at 37°C for 1-2 hours...HEK-293T cells that were inadvertently collected during harvesting. TIP: In lieu of centrifugation, you...based on your experiment Detailed protocols for preparing polybrene, protamine sulfate, and puromycin are...

  8. Video Library

    Type
    Protocol
    ...step-by-step walkthrough of Addgene's ordering process Ordering Page MTA FAQs Answers to frequently asked...Plates Create plates to culture bacteria in the lab Pouring LB Agar Plates Protocol Streaking Bacteria on Plates...enzymes Diagnostic Restriction Digest Protocol Storing and Handling Addgene Plasmids What to do after ...receive your plasmids from Addgene Instructions for Storing and Handling Plasmids Genomic Deletions with CRISPR...Australia, and advice for current graduate students considering their future careers. Eric J. Perkins, PhD In...

  9. AAV Production in HEK293 Cells

    Type
    Protocol
    ...~7.4. Autoclave or sterile filter. Pro-Tip Stirring during the cooling period is recommended or the solution...glucose, lower FBS media causes less filter clogging during harvesting. The addition of sorbitol has been shown...PEI powder into 100 mL of deionized water. While stirring, slowly add hydrochloric acid until the solution... challenging due to the high viscosity of PEG. Stirring under medium heat will promote faster dissolution...overgrow your cells. Pass the cells twice a week during the maintenance phase and do not allow cells to... °C for 1 h, then keep at 4 °C for 3 h without stirring to allow full precipitation. Precipitation of ...

  10. What is Polymerase Chain Reaction (PCR)

    Type
    Protocol
    ... of reagents and a basic heating and cooling (denaturing and annealing) cycle. The process became automated...in an appropriate buffer, a series of heating (denaturing) and cooling (annealing) steps allow the Taq ...template strand to the point where the strands start denaturing and the hydrogen bonds are broken between the... tops to the PCR tubes, gently tap each tube to bring all the liquid to the bottom before placing it in...sequence is GC-rich, increase the time of the denaturing. Your 5’ and 3’ primers should be designed to... that can withstand radical temperature changes during a typical PCR. The DNA polymerase has an optimum...

  11. Pipetting Protocol

    Type
    Protocol
    ...pipette shows the volume adjustment ring right below the plunger. This ring changes the pipette volume. Below... volume for the the pipette, and the tip ejector ring at the bottom which pushes the pipette tip off of...tip is so that the same pipette can be used for measuring different samples without cross contamination ...your fingers to avoid contaminating the tip or puncturing your glove. Ensure that the tip is properly set...

  12. AAV ddPCR Titration

    Type
    Protocol
    ... particular sample. For additional tips on AAV titering using ddPCR, read this blog post on ddPCR for ...all the way, just ensure the samples are covered. Bring the PCR tubes to the BSC used for dilutions. Without...Lightly cap the PCR tubes. Generate the Droplets Bring the PCR tubes to the droplet generation BSC. Without...samples on ice or pre-chilled 96-well freezer blocks during use. In this protocol, a dilution series is prepared...dilutions and titrations For additional tips on AAV titering using ddPCR, read our blog post. Last reviewed...

  13. DNA Quantification

    Type
    Protocol
    ...like... Inoculating a Liquid Bacterial Culture Recovering Plasmid DNA from Bacterial Culture Restriction...Restriction Digest of Plasmid DNA Background Information During several different stages of molecular cloning, ...specific wavelength that they maximally absorb. By measuring the absorbance of a liquid you can accurately ...specific to your lab. Spectrophotometer Tips Before measuring any samples, be sure to ‘blank’ the spectrophotometer...

  14. CRISPR Library Amplification

    Type
    Protocol
    ...as possible due to the inherent possibility of altering the composition of the library. Bottlenecks, fitness...representation of individual plasmids in the pooled library during amplification. This protocol is designed to be ...pulling motion Take care not to split or gouge agar during the scraping process. Add each scrape into a 50...efficiency! Ensure that no arcing is taking place during electroporation. Arcing would manifest as a loud... often accompanied by some light in the cuvette during the electroporation step. I got a heavy recombined...

  15. Protocols for Molecular Biology, Plasmid Cloning, and Viral Preps

    Type
    Protocol
    ... basic molecular biology, plasmid cloning, and titering and testing your viral preparations. ...and analyzing your plasmids. Virus Protocols for titering and testing your virus preparations. Antibodies...polyethyenimine (PEI) transfection protocol Fluorescence Titering Assay for Lentivirus Quantify virus using fluorescence...fluorescence measurements Colony Formation Titering Assay for Lentivirus Quantify virus by counting antibiotic...

  16. AAV Purification by Iodixanol Gradient Ultracentrifugation

    Type
    Protocol
    ...QuickSeal tube spacers 16 ga needle 18 ga needle 10 mL syringe 18 ga blunt edge needles, Hamilton 1X PBS pH 7.4...QuickSeal tube in the order below using a 10 mL syringe and a blunt edge 18 ga Hamilton needle, taking ...interface with an 18 ga needle attached to a 10 mL syringe. The bevel of the needle should be up, facing the... If the concentrate volume is less than 500 µL, bring up the volume with formulation buffer. Use a P1000...

  17. Protocol - How to Run an Agarose Gel

    Type
    Protocol
    ...bromide (stock concentration of 10 mg/mL) Procedure Pouring a Standard 1% Agarose Gel: Measure 1 g of agarose...the solution heats up.). Caution HOT! Be careful stirring, eruptive boiling can occur. Pro-Tip It is a good...on the sample to prevent bubbles or buffer from entering the tip. Place the very top of the tip of the ...Note: When using UV light, protect your skin by wearing safety goggles or a face shield, gloves and a lab...

  18. Affinity Purification of Recombinant Antibodies with Protein A or Protein G

    Type
    Protocol
    ...Protein A or Protein G columns. Sharing speeds science. We believe that sharing the full details of our protocols...89039-656 Microcentrifuge tubes, VWR 89126-724 Filtering system 0.2 µm PES, VWR 431098 Sodium phosphate...filtration unit, 500 mL, rapid-flow, VWR 73520-984 Syringes, 30 mL, VWR BD302832 Filter, 0.2 µm (luer-lock...

  19. Protocol - Over-Agar Antibiotic Plating

    Type
    Protocol
    ...Making LB Agar Plates Bacterial Transformation Recovering Plasmid DNA from Bacterial Culture Introduction... select transformed cells containing plasmids differing in their resistance genes, as one does not need... give the antibiotic time to more fully absorb. During the incubation, transform DH5α E. coli cells by...

  20. Molecular Biology Protocol - Restriction Digest of Plasmid DNA

    Type
    Protocol
    ...Restriction Digest of Plasmid DNA You may also like... Recovering Plasmid DNA from Bacterial Culture Purifying ...enzyme digestion takes advantage of naturally occurring enzymes that cleave DNA at specific sequences....Buffer 3 µL 10x BSA (if recommended) x µL dH 2 O (to bring total volume to 30µL) The amount of restriction ...
Showing: 1 - 20 of 48 results