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Plasmid Miniprep Kit II

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Plasmid Miniprep Kit II
Features :
Price : $10.00
Quantity :
Catalogue#: PD1213-00
  
 

Description :

Introduction

Key to the kit is our proprietary DNA binding systems that allow the high efficient binding of DNA to our ezBindTM matrix while proteins and other contaminates are removed under certain optimal conditions. Nucleic acids are easily eluted with sterile water or Elution Buffer.

This kit is designed for fast and efficient purification of plasmid DNA from 1 to 15 mL of E. coli culture. With the binding capacity of 80 ?g, the yield obtained by Miniprep Kit II (PD1213) is higher than Miniprep Kit I (PD1211). ?The yield from 1 mL culture is typically around 8 to 12 ?g. ?

The purified DNA is ready for downstream applications such as cloning/subcloning, RFLP, sequencing, and transfection of HEK293 cells.

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Important Notes

Plasmid Copy Numbers: 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 reference Table 1 for the commonly used plasmids,

Table 1 commonly used plasmid and expected yield.

Plasmid

Origin

Copy Numbers

Expected Yield(?g per 1 mL)

pSC101

pSC101

5

0.1-0.2

pACYC

P15A

10-12

0.4-0.6

pSuperCos

pMB1

10-20

0.4-1

pBR322

pMB1

15-20

0.6-1

pGEMR

Muted pMB1

300-400

6-7

pBluescriptR

ColE1

300-500

6-8

pUC

Muted pMB1

500-700

8-12

Host Strains: The strains used for propagating plasmid have significant influence on yield. Host strains such as Top 10 and DH5a yield high-quality plasmid DNA. endA+ strains such as JM101, JM110, HB101, TG1 and their derivatives, normally have low plasmid yield due to either endogenous endonucleases or high carbohydrates released during lysis. We recommend transform plasmid to an endA- strain if the yield is not satisfactory.

Table2 endA- strains of E. Coli.

EndA- Strains of E. Coli

DH5α

DH1

DH21

JM106

JM109

SK2267

SRB

XLO

TOP10

DH10B

JM103

JM107

SK1590

MM294

Stbl2TM

XL1-Blue

BJ5182

DH20

JM105

JM108

SK1592

Select96TM

Stbl4TM

XL10-Gold

EndA+ Strains of E. Coli

C600

JM110

RR1

ABLE? C

CJ236

KW251

P2392

BL21(DE3)

HB101

TG1

TB1

ABLE? K

DH12STM

LE392

PR700

BL21(DE3)pLysS

JM101

JM83

TKB1

HMS174

ES1301

M1061

Q358

BMH 71-18

All NM ?strains

All Y strains

Optimal Cell Mass (OD600 x mL of Culture): This procedure is designed for isolating plasmid grown in standard LB medium (Luria Bertani) for 12 -16 hours to a density of OD600 2.0 to 3.0. If rich mediums such as TB or 2xYT are used, make sure the cell density doesn't exceed 3.0 (OD600). A high ratio of biomass over lysis buffers result in low DNA yield and purity. The mini column has an optimal biomass of 30-45. For example, if the OD600 is 3.0, the optimal culture volume should be 10-15 mL. For over amount of cell numbers, either reduce the biomass or scale up the volumes of Buffer A1, B1 and N1.

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Culture Volume: Use a flask or tube 4 times bigger in volumn thanthe culture medium to secure optimal condition for bacteria growth. Don't exceed the maximum culture volume suggested in the protocol. Incomplete lysis due to over amount of bacterial culture results in lower yield and less purity.

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Storage and Stability

Buffer A1 should be stored at 4?C once RNase A is added. All other materials can be stored at room temperature (22-25?C). The Guaranteed shelf life is 12 months from the date of purchase.

Before Starting

Prepare all components and get all necessary materials ready by examining this instruction booklet and become familiar with each steps.

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Important

  • RNase A: It is stable for more than half a year when stored at room temperature. Spin down RNase A vial briefly. Add the RNase A solution to buffer A1 and mix well before use. Store at 4?C.
  • Add 8 mL (PD1213-00) or 60 mL (PD1213-01) or 60 mL (PD1213-02) or 96 mL (PD1213-03) 96-100% ethanol to each DNA Wash Buffer bottle before use.
  • Buffer B1 precipitates below room temperature. It is critical to warm up the buffer at 50?C to dissolve the precipitates before use.
  • Keep the cap tightly closed for Buffer B1 after use.
  • Ensure the availability of centrifuge capable of 13,000 rpm.
  • Carry out all centrifugations at room temperature.

Materials supplied by users

  • 96-100% ethanol
  • 1.5 mL, 2.0 mL microcentrifuge tubes.
  • 15 mL conical tubes.
  • High speed microcentrifuge or Vacuum manifold.

Kit Contents

Catalog#

PD1213-00

PD1213-01

PD1213-02

PD1213-03

Preps

4

50

100

250

ezBind Columns

4

50

100

250

Buffer A1

2.5 mL

25 mL

50 mL

125 mL

Buffer B1

2.5 mL

25 mL

50 mL

125 mL

Buffer N1

3 mL

30 mL

60 mL

135 mL

Buffer KB

3 mL

30 mL

60 mL

135 mL

DNA Wash Buffer*

2 mL

15 mL

2 x 15 mL

3 x 24 mL

Elution Buffer

1 mL

15 mL

30 mL

60 mL

RNase A (20 mg/mL)

0.25 mg(12.5 ?L)

2.5 mg(125 ?L)

5 mg(250 ?L)

12.5 mg(625 ?L)

User Manual

1

1

1

1

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*Add 8 mL (PD1213-00) or 60 mL (PD1213-01) or 60 mL (PD1213-02) or 96 mL (PD1213-03) 96-100% ethanol to each DNA Wash Buffer bottle before use.

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Safety Information

  • Buffer N1 contains acidic acid, wear gloves and protective eyewear while handling.
  • Buffer N1 and KB contains chaotropic salts, which may form reactive compounds when combines with bleach. Do not add bleach or acidic solutions directly to the preparation waste.

Operating Protocol

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