Kit de minipreparación de plásmidos PureLink™ Quick

Citas y referencias (4)

Invitrogen™

Kit de minipreparación de plásmidos PureLink™ Quick

Name: Kit de minipreparación de plásmidos PureLink™ Quick
SKU: K210010
Price: 101.980 CLP

El kit de minipreparación de plásmidos PureLink™ Quick se ha diseñado para un rápido aislamiento del ADN plasmídico de secuenciaciónMás información

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Número de catálogo	N.º de reacciones
K210010	50 preparaciones
K210011	250 preparaciones

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Número de catálogo K210010

Precio (CLP)

101.980

Each

Añadir al carro de la compra

N.º de reacciones:

50 preparaciones

Precio (CLP)

101.980

Each

Añadir al carro de la compra

El kit de minipreparación de plásmidos PureLink™ Quick se ha diseñado para un rápido aislamiento del ADN plasmídico de secuenciación de E. coli en entre 30 y 45 minutos, mediante columnas de membrana de sílice. Características del kit de minipreparación de plásmidos PureLink™ Quick:

• Rápido: ADN plasmídico listo para su uso normalmente en entre 30 y 45 minutos
• Flexible: formatos que funcionan con plataformas de vacío y centrifugación

Aislamiento fiable y económico de ADN plasmídico
El kit de minipreparación de plásmidos PureLink™ Quick permite aislar ADN plasmídico de gran calidad a partir de cultivos de 1 a 5 ml entre 30 y 45 minutos, mediante las columnas de centrifugación PureLink™. Estas columnas usan una exclusiva membrana de sílice para lograr una elevada producción de hasta 40 µg de ADN plasmídico de secuenciación. Las células se lisan mediante un procedimiento alcalino/SDS y el lisado se aplica a una columna de membrana de sílice que une selectivamente el ADN plasmídico. Los contaminantes se eliminan con el tampón de lavado y el ADN plasmídico se eluye en el tampón de TE. El ADN eluido es adecuado para todas las aplicaciones posteriores rutinarias.

Compatible con formatos flexibles
El kit de minipreparación de plásmidos PureLink™ Quick se puede utilizar con un colector de vacío o centrifugación para purificar ADN plasmídico. Por lo general, el ADN aislado mediante el kit de minipreparación de plásmidos PureLink™ Quick tiene un A₂₆₀/A₂₈₀ > a 1,80 cuando las muestras se diluyen en Tris-HCl (pH 7,5), lo que indica que el ADN está razonablemente libre de proteínas que podrían interferir con aplicaciones posteriores.

El ADN aislado se puede utilizar para diversas aplicaciones posteriores
El ADN plasmídico purificado mediante el kit de minipreparación de plásmidos PureLink™ Quick es adecuado para todas las aplicaciones posteriores rutinarias, como transformaciones de células de mamíferos y bacterianas, secuenciación de ADN, digestión de enzimas de restricción, clonación y PCR.

Para uso exclusivo en investigación. No apto para uso en procedimientos diagnósticos.

Especificaciones

Tipo de columnaColumna de centrifugación

Concentración20mg/ml

Tipo de producto finalADN plasmídico

Para utilizar con (aplicación)Secuenciación de última generación, clonación, secuenciación, etiquetado de ácidos nucleicos, PCR, transformación

Compatibilidad de alto rendimientoNo compatible con alto rendimiento (manual)

N.º de reacciones50 preparaciones

Escala preparativa<100 µ g de ADN plasmídico (pequeña escala)

Línea de productosPureLink

Tipo de productoKit de minipreparación de plásmidos Quick

Cantidad50 preparaciones

Tipo de muestraCultivo bacteriano

Condiciones de envíoTemperatura ambiente

ObjetivoADN plasmídico

Tiempo de pruebaDe 30 min a 45 min

FormatoColumna de centrifugación

Isolation TechnologyColumna de centrifugación de sílice

Unit SizeEach

Contenido y almacenamiento

• Resuspension buffer
• RNase A (20 mg/mL)
• Lysis buffer
• Precipitation buffer
• Wash buffers
• TE buffer
• Spin columns in wash tubes
• Elution tubes

Preguntas frecuentes

I'm getting low/no plasmid DNA after purification using a PureLink HiPure kit, even though there was measurable absorbance. Do you have any suggestions for what I can do?

A common problem encountered with absorbance measurements is turbidity of samples. (This could be caused by residual resin from the column.) If there is insoluble material in the cuvette (not often detected by the naked eye), much of the UV light is not absorbed but scattered, leading to an artificially high UV absorbance reading (at 260 or 280 nm, for example.) If your A260 is high, we recommend that you check the A320 to determine if there is resin in the sample. You can also try to centrifuge or filter (0.2 µm filter) your sample to remove any resin and then recheck the concentration.

I've run out of buffer when using the PureLink HiPure Plasmid Purification Kit (Cat. No. K210018). Can I purchase the buffers separately?

Yes, we would recommend purchasing the PureLink HiPure BAC Buffer Kit (Cat. No. K210018). This kit includes Resuspension Buffer (R3) (250 ml), Lysis Buffer (L7) (250 ml), Precipitation Buffer (N3) (250 ml), and RNase A (20 µg/ml) (5 ml).
You will need to add less RNase A than stated on the bottle label of the R3 buffer in this kit. It says to add 5.6 mL of RNase A. This is the correct amount for the BAC protocol; however, if you are performing standard plasmid isolation, 1.4 mL RNase A should be added.

Plasmid DNA isolated using a PureLink column-based purification kit from an endA+ strain is degraded after a restriction digest. Do you have a suggestion for this?

The HiPure kits should remove all protein from the DNA including endonucleases. For the silica-based PureLink Quick Plasmid Miniprep Kit, we recommend an extra wash with the optional Wash Buffer W10 to remove endonucleases. This solution is not compatible with the HiPure system and should not be used with those kits. Alternatively, heat the eluted DNA in TE for 10 min at 70 degrees C. This should heat-inactivate any contaminating nucleases.

I'm seeing extra bands present after plasmid purification using your PureLink column-based system. What could cause this to happen?

Extra bands can occur when plasmid DNA is nicked and/or permanently denatured. Plasmid DNA that has been nicked (covalently opened) will run slower than supercoiled DNA during electrophoresis. A small amount of this species of DNA is common and is suitable for downstream applications. Permanently denatured DNA will migrate ahead of the supercoiled DNA and may not be suitable for downstream applications. Do not allow the lysis reaction to proceed longer than 5 minutes.

My purified DNA has particles in it after column-based plasmid purification. Any suggestions?

We have seen this on occasion. The particles do not affect quality of the DNA. Remove the particles by performimg a 1 minute centrifugation at 12,000 x g.

View all Kit de minipreparación de plásmidos PureLink™ Quick FAQs

Citations & References (4)

Citations & References

Abstract

The refolding of different alpha-fetoprotein variants.

Authors:Leong SS, Middelberg AP,

Journal:Protein Sci

PubMed ID:16882993

The effect of glycosylation on AFP foldability was investigated by parallel quantitative and qualitative analyses of the refolding of glycosylated and nonglycosylated AFP variants. Both variants were successfully refolded by dialysis from the denatured-reduced state, attaining comparable ... More

Identification and cardiotropic actions of sulfakinin peptides in the American lobster Homarus americanus.

Authors:Dickinson PS, Stevens JS, Rus S, Brennan HR, Goiney CC, Smith CM, Li L, Towle DW, Christie AE,

Journal:J Exp Biol

PubMed ID:17575033

In arthropods, a group of peptides possessing a -Y((SO3H))GHM/LRFamide carboxy-terminal motif have been collectively termed the sulfakinins. Sulfakinin isoforms have been identified from numerous insect species. In contrast, members of this peptide family have thus far been isolated from just two crustaceans, the penaeid shrimp Penaeus monodon and Litopenaeus vannamei. ... More

Streptococcus iniae capsule impairs phagocytic clearance and contributes to virulence in fish.

Authors:Locke JB, Colvin KM, Datta AK, Patel SK, Naidu NN, Neely MN, Nizet V, Buchanan JT,

Journal:J Bacteriol

PubMed ID:17098893

Surface capsular polysaccharides play a critical role in protecting several pathogenic microbes against innate host defenses during infection. Little is known about virulence mechanisms of the fish pathogen Streptococcus iniae, though indirect evidence suggests that capsule could represent an important factor. The putative S. iniae capsule operon contains a homologue ... More

Sensitive multiplex real-time reverse transcription-PCR assay for the detection of human and animal noroviruses in clinical and environmental samples.

Authors:Wolf S, Williamson WM, Hewitt J, Rivera-Aban M, Lin S, Ball A, Scholes P, Greening GE,

Journal:Appl Environ Microbiol

PubMed ID:17616614

In this study, we developed a triplex real-time reverse transcription-PCR (RT-PCR)-based method that detects and distinguishes between noroviruses belonging to genogroups I, II, and III and that targets the junction between the regions of open reading frame 1 (ORF1) and ORF2. This is the first assay to include all three ... More