Phage DNA Isolation Kit
For the rapid purification of total DNA from bacteriophages.
For research use only and NOT intended for in vitro diagnostics.
For the rapid purification of total DNA from bacteriophages.
For research use only and NOT intended for in vitro diagnostics.
For the rapid purification of total DNA from bacteriophages.
Register today to receive an exclusive 15% off* on your first order.
This kit provides a rapid spin column method for the purification of total DNA from a broad spectrum of bacteriophages propagated in bacteria grown in liquid cultures. The DNA is isolated without the use of phenol, chloroform or cesium chloride banding procedures. The spin-column based procedure is rapid and can be completed in less than 45 minutes. The kit is highly efficient for processing small volumes of phage supernatant (500 µL – 1 mL) and with the optional DNase and Proteinase K treatments phage DNA yields are maximized while host DNA contamination is minimized. Purified total phage DNA is of the highest integrity, and can be used in a number of downstream applications including PCR, qPCR, Restriction Fragment Length Polymorphism (RFLP), sequencing, cloning, Southern Blot and more.
Kit Specifications
|
|
Column Binding Capacity
|
50 µg
|
Maximum Column Loading Volume
|
650 µL
|
Size of DNA Purified
|
All sizes
|
Maximum Amount of Starting Material |
1 x 1010 pfu/mL enriched phages
|
Average Yield* |
3-15 µg DNA from 108-1010 pfu/mL
of enriched phages |
Time to Complete 10 Purifications |
45 minutes
|
* Average yields will vary depending upon a number conditions used and developmental stage.
Storage Conditions and Product Stability
All solutions should be kept tightly sealed and stored at room temperature. This kit is stable for 1 year after the date of shipment.
Component | Cat. 46800 (50 preps) | Cat. 46850 (100 preps) |
---|---|---|
Lysis Buffer B | 40 mL | 2 x 40 mL |
Wash Solution A | 38 mL | 2 x 38 mL |
Elution Buffer B | 8 mL | 2 x 8 mL |
Spin Columns | 50 | 100 |
Collection Tubes | 50 | 100 |
Elution Tubes (1.7 mL) | 50 | 100 |
Product Insert | 1 | 1 |
Column clogging may occur due to one or more of the following reasons:
Check the centrifuge to ensure that it is capable of generating the required RPMs. Sufficient centrifugal force is required to move the liquid through the resin. Also, ensure that the correct spin times are followed. Spin for an additional minute if necessary.
Ensure that the starting material is clarified phage supernatant. Remove bacterial debris from the initial phage supernatant by centrifugation at 10,000 × g for 5 minutes before beginning the protocol.
To ensure a homogeneous solution, vortex for 10-15 seconds before applying the lysate to the spin column.
Ensure that the centrifuge remains at room temperature throughout the procedure. Temperatures below 20℃ may cause precipitates to form that can cause the columns to clog.
The yield of genomic DNA may be lower than expected due to the following:
Refer to the manufacturer's recommendations for the propagation of the phage, including proper titer for inoculation, growth conditions, and bacterial host.
Ensure that the incubation was performed for 15 minutes at 65℃ after the addition of Lysis Buffer B. Also, perform optional digestion with Proteinase K in Step 1b during Lysate Preparation.
Ensure that 90 mL of 96 - 100% ethanol is added to the supplied Wash Solution A prior to use.
Ensure that all the DNA is eluted. If elution buffer remains in the column, use 14,000 g for the second centrifuge.
If the DNA does not perform well in downstream applications, it may be due to one or more of the following:
Traces of salt from the binding step may remain in the sample if the column is not washed three times with the Wash Solution A. Salt may interfere with downstream applications and thus must be washed from the column.
Ensure that the dry spin under the Column Wash procedure is performed in order to remove traces of ethanol prior to elution. Ethanol is known to interfere with many downstream applications.
Host genomic DNA can contaminate the phage DNA. In order to eliminate host genomic DNA contamination in the phage DNA elution, it is recommended that a DNase I treatment is performed at the beginning of the lysate preparation procedure (see Section 1, Optional DNase Treatment).
Yes, the kit can isolate both ssDNA and dsDNA phage genomes.
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Authors | Hongmei Yin | Jinli Wang | Likou Zou | Anjian Liang | Chenglin Zhu | Yu Fu | Juan Chen | Junni Tang |
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Title | A gradient phage-assisted continuous evolution method for screening suppressor tRNAs in Escherichia coli |
Citation | New Biotechnology 2024. |
Authors | Fan Wang a b 1, Li-Hua Liu b c 1, Zhenyu Wang a 1, Ao Jiang b 1, Yi-Rui Wu |
Title | Discovery and characterisation of new phage targeting uropathogenic Escherichia coli |
Citation | Prepriint BIORXIV 2024. |
Authors | Shahla Asgharzadeh Kangachar1 , Dominic Y. Logel2,3, Ellina Trofimova2,3, Hannah X Zhu2,3, Julian Zaugg1 , Mark A. Schembri4,5, Karen D. Weynberg1 , Paul R. Jaschke2,3* |
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Citation | Microbiology Resource Announcements 2024. |
Authors | Evan B. Harris,1 Laura B. Anthony,1 Sakhawat Ali,1 Hannah Atkin,1 Lucy C. Bowden,1 Steven W. Brugger,1 Emille L. Carr,1 Nathaniel Eberhard,1 Samuel Flor,1 Rochelle K. Gaertner,1 Austen Gleave,1 David Hess,1 Trevor Hoggan,1 Elisa Correa Lazaro,1 Katherine Leonard,1 Trek Lewis,1 Colleen R. Newey,1 Joshua Ramsey,1 Kayla R. Sajous,1 Daniel Schaeffer,1 Tyson Stoker,1 Sierra Stump,1 Daniel W. Thompson,1 Rachel Weyland,1 Julianne H. Grose1 |
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Authors | Christopher J. Kovacs 1,2,Erika M. Rapp 1,William R. Rankin 1,Sophia M. McKenzie 1,Brianna K. Brasko 1,Katherine E. Hebert 1,Beth A. Bachert 1ORCID,Andrew R. Kick 1ORCID,F. John Burpo 1ORCID andJason C. Barnhill |
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Citation | scientific reports 2024. |
Authors | Characterization of two novel Salmonella phages having biocontrol potential against Salmonella spp. in gastrointestinal conditions |