[PM6628] ProMetric™ TriColor Low Range Protein Ladder, 2 to 40 kDa, 250 μl

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Description 

The PM6628 ProMetric™ TriColor Low Range Protein Ladder, 2 to 40 kDa, is a ready-to-use three-color protein standard with 6 pre-stained proteins covering a range of molecular weights from 2 to 40 kDa. Proteins are covalently coupled with a blue chromophore except for two reference bands (one green and one red band at 10 kDa and 40 kDa respectively) when separated on SDS-PAGE. The PM6628 ProMetric™ TriColor Low Range Protein Ladder is designed for monitoring protein separation during SDS-PAGE electrophoresis, verification of Western transfer efficiency on membranes (PVDF or nitrocellulose) and for approximating the molecular weight of small proteins.


Features

Ready-to-use — Premixed with a loading buffer for direct loading, no need to boil

Two reference bands — 40 kDa (red) and 10 kDa (green)

Enhanced band clarity for proteins below 10 kDa

Versatile application across various gel systems, including Tris-Tricine, Tris-Glycine, and Bis-Tris gels


Storage Buffer

20 mM Tris-phosphate (pH 7.5 at 25°C), 1% SDS, 6 M Urea, and 20% (v/v) DMSO.


Quality Control

Under suggested conditions, PM6628 ProMetric™ TriColor Low Range Protein Ladder, 2 to 40 kDa, resolves 6 major bands in SDS-PAGE (Tris-tricine-SDS Buffer).


Storage

4°C for 3 months

-20°C for long term storage



 

Specification


Cat. No.

PM6628

Series Name

ProMetric™

Product Size

250 μl

MW Range

2 – 40 kDa

Band Number 6

6

Band Color  

Red/Green/Blue

Markered Bands

10, 40 kDa



Manual

Manual_PM6628_ProMetric™ TriColor Low Range Protein Ladder (2024 ver. 1.1.0)  

SDS

SDS_PM6628


Migration patterns and approximate MWs (kDa).




Tips for usage

1.Optimal gel conditions for PM6628:

  • For optimal results with the PM6628, we recommend using a 37.5:1 or 29:1 acrylamide-to-bisacrylamide ratio for Tris-Tricine gels. 

  • Avoid the 19:1 ratio due to its variability in formulation, potential use of hazardous chemicals, and longer electrophoresis times, particularly with 18% Tricine gels. 

  • Using Tris-Tricine gels with concentrations in the range of 14% to 16% is generally sufficient to achieve good separation of the PM6628.


2.Tips for separating low MW proteins (e.g., < 10 kDa) using Tris-Glycine gels:

  • Opt for a 15% acrylamide gel: In Tris-Glycine gel electrophoresis, a 15% acrylamide gel is generally effective for separating small proteins in the 2 to 10 kDa range.

  • Using higher acrylamide concentrations: Gels with acrylamide concentrations higher than 15% may show decreased resolution for small proteins due to challenges in gel preparation, such as uneven polymerization and bubble formation. If using a higher acrylamide gel is necessary, consider the following tips:

a. Keep stacking gel layer thin: Limit the stacking gel layer to less than 5 mm (from the well bottom to the top of the separation layer) to ensure proper stacking and avoid ambiguous results.

b. Adjust electrophoresis setting: For better stacking of small proteins, try running the electrophoresis at 100V for 15 minutes followed by 150V for 60 minutes.

c. Use a loading tip: Employ a gel loading tip to accurately load samples and protein markers near the well bottom, which helps to improve stacking and separation of very small proteins.


3.Tips for Western Blotting of low molecular weight proteins:

  • Choose appropriate membrane:  

Use membranes with smaller pore sizes (e.g., 0.2 μm) for better transfer of small proteins. Thicker PVDF membranes enhance binding and stability. Consider using NC membranes, if your target proteins or peptides are prone to be lost on PVDF.

  • Optimize transfer buffer:  

Avoid adding SDS to the transfer buffer as it impairs protein binding. Increase methanol concentration up to 25% for better membrane binding. Alternatively, using ethanol can also enhance binding for small proteins.

  • Post-transfer procedure:  

Rinse the membrane with distilled water immediately after transfer. Proceed with blocking, washing, and incubation at 4°C. If further immobilization of small peptides on membrane is needed, dry the membrane at room temperature before blocking. Limit Tween-20 to no more than 0.1% in washing and blocking buffers.



 

 

 

To be update


 

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