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Elispot MultiScreen®HTS Filter Plates and Antibody Pairs

Elispot MultiScreen®HTS Filter Plates demonstrate improved spot recovery and spot definition

Related Resources

Overview

Specifications

Ordering Information

MultiScreenHTS Filter PlatesClear Sorting & Filtering Show Filter
Catalogue NumberDescriptionChemistrySterilityDevice MaterialColor CodePack Size
MSIPS4W10MultiScreenHTS IP Filter Plate, 0.45 µm, white, sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Sterile Acrylic White 10 Show Pricing & Availability
MSIPN4W50MultiScreenHTS IP Filter Plate, 0.45 µm, white, non-sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Non-Sterile Acrylic White 50 Show Pricing & Availability
MSIPN4550MultiScreenHTS IP Filter Plate, 0.45 µm, clear, non-sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Non-Sterile Acrylic Clear 50 Show Pricing & Availability
MSIPS4510MultiScreenHTS IP Filter Plate, 0.45 µm, clear, sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Sterile Acrylic Clear 10 Show Pricing & Availability

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MultiScreen Filter PlatesClear Sorting & Filtering Show Filter
Catalogue NumberDescriptionChemistrySterilityDevice MaterialColor CodePack Size
MAIPS4510MultiScreen-IP Filter Plate, 0.45 µm, clear, sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Sterile Acrylic Clear 10 Show Pricing & Availability
S2EM004M99MultiScreen-IP Filter Plate, 0.45 µm, white, sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Sterile Acrylic White 10 Show Pricing & Availability
MAIPSWU10MultiScreen-IP Filter Plate w/o underdrain, 0.45 µm, white, sterile Hydrophobic Polyvinylidene Fluoride (PVDF) Sterile Acrylic White 10 Show Pricing & Availability
MAHAS4510MultiScreen-HA Filter Plate, 0.45 µm, clear, sterile Mixed Cellulose Esters (MCE) Sterile Styrene Clear 10 Show Pricing & Availability

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Documentation

References

Reference overviewApplication
Simultaneous detrection of multiple cytokines in ELISPOT assays.
Palzer S. Bailey T., Hartnett C., Grant A., Tsang M., Kalyuzhny AE.
Methods Mol Biol. 2005; 305:273-88  2005

ELISPOT Assays
The Granzyme B ELISPOT assay: an alternative to the 51Cr-release assay for monitoring cell-mediated cytotoxicity
Kimberly Shafer-Weaver, Thomas Sayers, Susan Strobl, Eric Derby, Tracy Ulderich, Michael Baseler and Anatoli Malyguine
Journal of Translational Medicine 2003, 1:14     doi:10.1186/1479-5876-1-14  2003

ELISPOT Assays
Protein kinase C [beta]II activation induces angiotensin converting enzyme expression in neonatal rat cardiomyocytes.
Yuke Zhang, Laura J. Bloem, Lan Yu, Thomas B. Estridge, Philip W. Iversen, Christine E. McDonald, James P. Schrementi, XuShan Wang, Chris J. Vlahos and Jian Wang
Cardiovascular Research 57 (1): 139-146  2003

Enzyme Assays
Regional, but not systemic recruitment/expansion of dendritic cells by a pluronic-formulated Flt3-ligand plasmid with vaccine adjuvant activity.
Hongxun Sang, Vladimir M. Pisarev, Corey Munger, Simon Robinson, Jennifer Chavez, Lori Hatcher, Prahlad Parajuli, Yajun Guo and James E. Talmadge
Vaccine 21 (21-22): 3019-3029  2003

ELISPOT Assays
CD40 ligand (CD154) improves the durability of respiratory syncytial virus DNA vaccination in BALB/c mice.
Jennifer L. Harcourt, Michael P. Brown, Larry J. Anderson and Ralph A. Tripp
Vaccine 21 (21-22): 2964-2979  2003

ELISPOT Assays
Rectal immunization of mice with hepatitis A vaccine induces stronger systemic and local immune responses than parenteral immunization.
Leslie Ann Mitchell and Eithan Galun
Vaccine 21 (13-14): 1527-1538  2003

ELISPOT Assays
A novel multivalent human CTL peptide construct elicits robust cellular immune responses in HLA-A*0201 transgenic mice: implications for HTLV-1 vaccine design.
Roshni Sundaram, Yiping Sun, Christopher M. Walker, Francois A. Lemonnier, Steven Jacobson and Pravin T. P. Kaumaya
Vaccine 21 (21-22): 2767-2781  2003

ELISPOT Assays
Effective induction of CD8+ T-cell response using CpG oligodeoxynucleotides and HER-2/neu-derived peptide co-encapsulated in liposomes.
Wai Ming Li, Wieslawa H. Dragowska, Marcel B. Bally and Marie-Paule Schutze-Redelmeier
Vaccine 21 (23): 3319-3329  2003

ELISPOT Assays
The role of lipopolysaccharide in T-cell responses following DNA vaccination.
William G. Hawkins, Jiri Trcka, Neil Segal, Nathalie E. Blachere, Jason S. Gold, Yoichi Moroi, Wilbur B. Bowne, Jonathan J. Lewis, Jedd D. Wolchok and Alan N. Houghton
Vaccine 21 (13-14): 1548-1553  2003

ELISPOT Assays
A quantitive, highly sensitive cell-based infectivity assay for mouse scrapie prions.
P.-C. Klöhn, L. Stoltze, E. Flechsig, M. Enari, and C. Weissmann
PNAS 100 (D6920): 11666-11671  2003

ELISPOT Assays

FAQ

QuestionAnswer
When performing an ELISpot assay should MultiScreen plates with Immobilon-P membrane (MAIP and MSIP) be initially pre-wet with alcohol(methanol/ethanol)?Yes. Wetting the membrane with 15 µL alcohol followed by two to three washes with sterile PBS will allow the antibody more intimate contact with the membrane. Do not vacuum the alcohol through the underdrain, rather it should be flicked out. Once the membrane is pre-wet with alcohol, do not allow it to dry for the duration of the assay.
Should MultiScreen MAHA and MSHA ELISpot plates with MCE membranes be initially pre-wet with alcohol or sterile buffer?No. Neither is necessary. Methanol will dissolve the mixed-cellulose ester membrane. PBS is no longer needed. Membrane improvements ensure instant wetting of the membrane.
We are looking to coat MultiScreen ELISpot plates with primary antibody and store them. Do you have a recommended protocol?After coating with primary antibody overnight at 4°C, wash twice with 150µL sterile Milli-Q® water. Dry plates thoroughly under sterile conditions and store for up to one week at 4°C. If longer storage is desired, the plates should be washed as previously described and then blocked (150µL/well media, 37°C, 2hr). Following blocking, wash 2x with 150µL sterile Milli-Q. Dry as before and store desiccated. Ab activity may diminish over time - especially in the event that the plates have not been blocked. Millipore has not determined shelf-life for either protocol as performance stability is likely to depend largely on the properties of the specific antibody under investigation.