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EP951032921

Eppendorf® Deepwell plates, Protein LoBind, 96 wells

yellow plate, conical bottom, colorless wells, capacity 500 μL, pkg of 20 ea (5 bags × 4 plates)

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About This Item

UNSPSC Code:
41106300
Material:
clear wells, colorless wells, conical bottom, polypropylene , yellow plate
Size:
96 wells
Sterility:
non-sterile
Binding type:
low binding surface
Feature:
lid: no

Key Documents

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size

96 wells

binding type

low binding surface

material

clear wells, colorless wells, conical bottom, polypropylene , yellow plate

sterility

non-sterile

feature

lid: no

packaging

pkg of 20 ea (5 bags × 4 plates)

manufacturer/tradename

Eppendorf® 951032921

capacity

500 μL

well volume

1000 μL

color

yellow border

suitability

suitable for (protein analysis), suitable for PCR

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General description

Deepwell Plate 96/1000 µL, Protein LoBind, wells colorless, 1,000 µL, PCR clean, yellow, 20 plates (5 bags × 4 plates)
  • Eppendorf LoBind material ensures excellent sample recovery for improved assay results
  • Free of surface coating (e.g., silicone) to minimize the risk of sample interference
  • Lot-certified PCR clean purity grade: free of human DNA, DNase, RNase and PCR inhibitors
  • Available in tube, microplate, and deepwell plate formats for easy-up scaling
  • Unique OptiTrack® matrix: 30 % faster sample identification and fewer pipetting errors
  • RecoverMax well design: optimized well geometry for minimal remaining/dead volume and excellent mixing properties
  • Raised well rims and a smooth surface ensure reliable sealing in plates

Features and Benefits

  • Eppendorf LoBind material ensures optimized sample recovery for improved assay results
  • Free of surface coating (e.g. silicone) to minimize the risk of sample interference
  • Lot-certified PCR clean purity grade: free of human DNA, DNase, RNase and PCR inhibitors
  • Available in tube, microplate, and deepwell plate formats for easy-up scaling
  • High-contrast Unique OptiTrack® matrix: up to 30 % faster sample identification and fewer pipetting errors
  • RecoverMax® well design: optimized well geometry for minimal remaining/dead volume and excellent mixing properties
  • Raised well rims and a smooth surface ensure reliable sealing

Legal Information

Eppendorf is a registered trademark of Eppendorf SE
OptiTrack is a registered trademark of Eppendorf SE
RecoverMax is a registered trademark of Eppendorf SE

Regulatory Information

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Connie Luk et al.
Journal of neurochemistry, 123(3), 396-405 (2012-08-07)
Characteristic tau isoform composition of the insoluble fibrillar tau inclusions define tauopathies, including Alzheimer's disease (AD), progressive supranuclear palsy (PSP) and frontotemporal dementia with parkinsonism linked to chromosome 17/frontotemporal lobar degeneration-tau (FTDP-17/FTLD-tau). Exon 10 splicing mutations in the tau gene
Nikos Tsolakos et al.
Vaccine, 28(18), 3211-3218 (2010-03-02)
In this study, we evaluated the effect of the growth medium on the composition and immunogenicity of meningococcal outer membrane vesicle (OMV) vaccines after cultivation of the Norwegian serogroup B 44/76 vaccine strain in either Frantz' or modified Catlin-6 media
M Yang et al.
International journal of pharmaceutics, 331(2), 176-181 (2006-11-28)
Salmon calcitonin (sCT) powders suitable for inhalation, containing chitosan and mannitol as absorption enhancer and protection agent, respectively, were prepared using a spray-drying process. The effect of chitosan on physicochemical stability of sCT in the dry powder was investigated by
E I Trilisky et al.
Journal of chromatography. A, 1142(1), 2-12 (2007-01-24)
Purified viruses are used in gene therapy and vaccine production. Ion-exchange chromatography (IEC) is the most common method for large-scale downstream purification of viruses and proteins. Published IEC protocols provide details for specific separations but not general methods for selecting
Thandavarayan Kathiresan et al.
Methods in molecular biology (Clifton, N.J.), 493, 269-286 (2008-10-08)
Functional proteomics comprises a wide range of technologies for the identification of novel protein-protein interactions and biological markers. Studies of protein-protein interactions have gained from the development of techniques and technologies such as immunoprecipitation, preparative two-dimensional (2-D) gel electrophoresis for
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