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Introducción
ARNasa A is an endoribonuclease that specifically degrades single-stranded RNA at C and U residues. It cleaves the phosphodiester bond between the 5′-ribose of a nucleotide and the phosphategroup attached to the 3′-ribose of an adjacent pyrimidine nucleotide. The resulting 2′,3′-cyclic phosphate is hydrolyzed to the corresponding 3′-nucleoside phosphate. The highest activity is exhibited with single-stranded RNA. RNase A is a single chain polypeptide containing 4 disulfide bridges.
A major application for RNase A is the removal of RNA from preparations of ADN plásmido. The enzyme is active under a wide range of reaction conditions. At low salt concentrations (0 a 100 mm NaCl), RNase A cleaves single-stranded and double-stranded RNA as well as the RNA strand in RNA-DNA hybrids. Sin embargo, at NaCl concentrations of 0.3 M or higher, RNase A specifically cleaves single-stranded RNA.
Detalles
Especificaciones
Características | Especificaciones |
Pureza | ≥60% RNase A basis (Ficha de datos de seguridad (MSDS)-PÁGINA) |
Enzymatic activity | >50 Kunitz units/mg protein |
Optimum reaction temperature | 60°C (effective active temperature is 15-70°C) |
Condiciones de transporte | Normal temperature transportation |
Condiciones de conservación | -20-8°C, almacenamiento en seco, el almacenamiento a largo plazo debe realizarse a -20°C. |
Solicitud 1: adding in the extraction process | 1. Plasmid Extraction: add RNase A (25mg/ml) to buffer P1 with a final concentration of 100-300μg/ml.
2. Extracción de ADN: add RNase A (25mg/ml) to the digestion solution with a final concentration is 100-400μg/ml, mix well and place at room temperature for 10-15 minutos. when SDS/CTAB in lysate exceeds 2%, RNase activity will be significantly inhibited; guanidina salt(>4M guanidine hydrochloride or >3M isotiocianato de guanidina) also significantly inhibited RNase A. When RNase A is added to the lysate, the RNase digestion effect can be extracted by appropriately diluting to reduce the concentration of SDS, CTAB and guanidine salt. |
Solicitud 2: | 1. Remove RNA contamination from crude genomic DNA products: add DNase free RNase A (10mg/ml) to crude DNA products with a final concentration of 10-100μg/ml. Después de mezclar, lugar a temperatura ambiente para 10 minutos.
2. Remove RNA contamination from plasmid DNA products: add DNase free RNase A (10mg/ml) to crude DNA products with a final concentration of 10μg/ml. Después de mezclar, it can be directly used for sequencing at room temperature for 10 minutos. |
Información sobre pedidos
Contenido | C12123 | C12124 | C12128 | C12129 |
RNase A Solution (25mg/ml) | 10 ml | 100 ml | ||
DNase Free RNase A Solution (10mg/ml) | 10 ml | 100 ml |
Reseñas
Aún no hay reseñas.