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HBHPD 100 HBHPD 300
PD1 Buffer 30 ml 90 ml
PD2 Buffer 30 ml 90 ml
PD3 Buffer 40 ml 120 ml
PDW Buffer (concentrate) 35 ml 98 ml
Wash Buffer (concentrate) 20 ml 50 ml
Elution Buffer 15 ml 35 ml
PD Column 100 pcs 300 pcs
Collection Tube 100 pcs 300 pcs
RNase A (Lyophilized) 3 mg 9 mg
User Manual 1 1
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Specification:

  • Principle : spin column (silica matrix)
  • Sample size : 1 ~ 5 ml
  • Size of plasmid or construct : < 15 kb
  • Operation time : < 25 minutes
  • Typical Yield : 25 ~ 40 µg
  • Binding capacity : 60 µg/ column
  • Column applicability : centrifugation and vaccum

Important Notes:

  • Store RNase A at -20 °C upon recipit of kit.
  • Add 0.5 ml of PD1 Buffer to a RNase A tube, Dissolve the RNase A by vortexing. Briefly spin the tube and transfer the total RNase A mixture back to the PD1 bottle, mix well by vortexing and store the PD1 buffer at 4 °C.
  • If precipitates have formed in PD2 Buffer, warm the buffer in 37°C waterbath to dissolve precipitates.
  • Preparation of PDW Buffer and Wash Buffer by adding 96 ~100% ethanol (not provided) for first use.
  • Centrifugation steps are done by a microcentrifuge capable of the speed at 11,000 ~1,8000 x g.
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