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Biomiga 96-well Plasmid ezFilter Mini Kit - PD1812-00

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Description :

Introduction

The yield of plasmid DNA depends on the origin of the replication and the size of the plasmid. The protocols are optimized for high copy number plasmid purification. For low copy number plasmids, both the culture volume and the buffer volume need to be scaled up 3 to 5 times. Please contact our customer service for further information and reference the table below for the commonly used plasmids.

Plasmid

Origin

High copy

Low copy

pACYC

P15A

 

10-12

pSC101

pSC101

 

5

pSuperCos

pMB1

 

10-20

pBR322

pMB1

 

15-20

pUC

Muted pMB1

500-700

 

pGEMR

Muted pMB1

300-400

 

pBluescriptR

ColE1

300-500

 

 

Materials supplied by user

  •  Centrifuge with swing-bucket rotor (4,000 x g).
  •  Please disinfect 96-well 2.2 mL plates before use.
  •  Vacuum pump capable of achieving 300-400 mbar.
  •  Standard vacuum manifold.
  •  Oven or incubator preset to 70 oC.

Storage and Stability

All components are guaranteed for 24 months from the date of purchase. The Buffer A1/RNase A should be stored at 4oC.

Kit Contents

Catalog#

PD1812-S

PD1812-01

PD1812-02

Preps

1

4

20

96- Well 2.2 mLPlate

1

4

20

96- Well 1.6 mLPlate(Can be reused)

1

4

20

96-Well DNA Plate

1

4

20

96-Well Lysate Clearance Plate

1

4

20

96-Well Collection Plate

2

5

24

Ventilating Film

1

4

20

Sealing Film

4

16

80

Buffer A1

30 mL(Add RNase A before use)

110 mL(Add RNase A before use)

2 x 300 mL

Buffer B1

30 mL(Keep tightly capped after use)

110 mL(Keep tightly capped after use)

2 x 300 mL

Buffer N1

40 mL(Contain chaotropic salts)

160 mL(Contain chaotropic salts)

2 x 400 mL

DNA Wash Buffer

50 mL(Add 200 mL ethanol before use)

2×100 mL(Add 400 mL ethanol before use)

7 x125 mL(Add 500 mL ethanol before use)

Buffer KB

55 mL

240 mL

3 x 400 mL

Elution Buffer

25 mL

100 mL

450 mL

RNase A(20mg/mL)

160 μL

600 μL

2 x 1.5 mL

Use Manual

1

1

1

Before Starting

Exam this handbook and get familiar with each step. Prepare all components and have the necessary materials ready.

  •  Briefly spin down the RNase A vial and add the RNase A to Buffer A1.
  •  Dilute DNA Wash Buffer as follows:

PD1812-00: Add 200 mL 96-100% ethanol to each bottle before use.

PD1812-01: Add 400mL 96-100% ethanol to each bottle before use.

PD1812-02: Add 500mL 96-100% ethanol to each bottle before use.

Operating Protocol

                 


  • Model: PD1812-00
  • Manufactured by: Biomiga

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