SUNRESIN
Stock Code 300487
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Polymeric Chromatography Resins
Polymeric Chromatography Resins
Styrene/DVB
Styrene/DVB
Ion Exchange
Ion Exchange

Seplife® LXMS 30S

  • Highly uniform particle size for high resolution
  • Strong cation exchange resin based on a hydrophilic coated styrene/divinylbenzene backbone functionalized with sulphonate (S)
  • Suitable for ion exchange chromatography in the separation of proteins, peptides, oligonucleotides and other small and medium size biomolecules
  • Seplife® LXMS 30S is a polymeric resin for ion exchange chromatography characterized by strong chemical stability and high rigidity for use in polishing steps with or without organic solvents and at high flow rates.
    Seplife® LXMS 30S is polymeric resin for ion exchange chromatography based on styrene/divinylbenzene functionalized with sulphonate (S) with a highly uniform particle size (30 micron).
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Products

Properties

Product

Seplife® LXMS 30S

Appearance

White to light yellow spherical beads

Type

Strong acid cation-Sulfonic acid

Matrix

Polystyrene/divinylbenzene

Ligand

Sulfonic acid

Ion exchange capacity (mmol/ml)

0.07-0.10

Particle size range (μm)

27-30

Typical pore size (Å)

500

pH stability

2-12 (operation), 1-14 (CIP)

Chemical stability

Stable in commonly used aqueous ion exchange buffers

Flow rate* (cm/h)

Max 900

Dynamic binding capacity** (mg/ml)

≥90

Shipped as

Slurry in 20% ethanol solution

* Testing conditions: Chromatography column 16mm×200mm; Column bed height 100mm; Packing pressure 2 MPa; Mobile phase 0.5mol/L NaCl.

**Testing conditions: Chromatography column 8mm×100mm; Column bed height 100mm; Packing pressure 0.5 MPa,; Mobile phase: 20mmol/L PB buffer pH6.8; Sample: Lysozyme; Retention time 2 minutes.

 

Instructions

Column packing

The best column packing results are obtained with the resin slurry in 0.5M NaCl at a concentration of 60%-70%.

· Mix the resins to form a homogenate and measure the desired mass or volume, about 1.2 times the column volume.

· Replace 20% ethanol with 0.5 M NaCl solution and equilibrate overnight.

· Before loading the column, adjust the slurry concentration to 65-70% with 0.5 M NaCl solution; pour the resin slurry into the chromatography column in one go, allow to sediment by gravity and mark the height after sedimentation.

· Load the distributor and adjust the height so that the compression coefficient is 1.05-1.10; then pump 0.5M NaCl through the column and stabilize the bed with 1.5 to 2 times the highest working flow rate. (2 - 5 column volumes).

· Efficiency and asymmetry determinations can be performed as described below.

Column Efficiency Evaluation

The test method for column efficiency of the chromatography columns is as follows:

Mobile phase: 0.5 M NaCl solution

Linear flow rate: 100 cm/h

Sample: 2 M NaCl solution

Loading volume: 0.5-1% of column volume

Detection: conductivity detector

Acceptable column asymmetry factor is in the range 0.8-1.8.

Rinsing

The loaded columns should be rinsed with at least 5 BV of deionized water.

Equilibration

Equilibrate the column with an appropriate 5-10 column volume buffer until the conductivity and pH of the effluent remain unchanged.

Sample feeding

The solid sample can be prepared by dissolving in the equilibrium solution; the low concentration sample solution can be dialyzed by the equilibrium solution; the high concentration sample solution can be diluted by the equilibrium solution. To avoid clogging of the column, samples should be processed by centrifugation or membrane filtration. The feed amount is calculated according to the capacity of the resin and the content of the target protein in the feed solution. Before loading, make sure that the sample buffer should be as consistent as possible with the equilibration solution.

Elution

After loading the sample, continue rinsing with equilibration buffer until the baseline is stable. Typically, the molecules retained on the chromatographic media are eluted by increasing the salt concentration or changing the pH to ensure repulsion of the charged species. Occasionally, a solution containing a small percentage organic solvent such as acetonitrile or ethanol is required to disrupt any hydrophobic interactions.

Regeneration and CIP

Regular CIP can prevent the enrichment of protein precipitation impurities in the column bed, and help to maintain the capacity and separation effect of the chromatography media. In general, specific CIP methods and the frequency of CIP need to be designed for each process according to the type of contaminants. The recommended regeneration and CIP method is as follows: Rinse with 5 BV 1-2 M NaCl followed by 5 BV 0.5-1 M NaOH.

Storage

Sealed and stored at 4-30°C (storage solution is 20% ethanol) in a ventilated, dry and clean place, do not freeze. 

Ordering information

Product Name

References

Pack Size

Seplife® LXMS 30S

PS40123X(30)1-1

25ml

PS40123X(30)1-2

100ml

PS40123X(30)1-3

500ml

PS40123X(30)1-4

1L

PS40123X(30)1-5

5L

PS40123X(30)1-6

10L

Production date: See label

Expiry date: 5 years, under proper storage conditions

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