Technical Support

Common reasons for non-specific staining

Too much Pentamer for the number of cells

One test of Pentamer should stain 1-2 x 10⁶ antigen-specific cells. However, it is recommended that the Pentamer is titrated prior to use. Carry out a range of doubling dilutions from 1 test per 1 x 10⁶ cells down to 1/16 test per 1 x 10⁶ cells. This will solve most cases of non-specific Pentamer staining.

Pentamer was not centrifuged prior to staining

Labeled Pentamers and Fluorotags should be centrifuged at 14000 rpm for 3-5 minutes to isolate any aggregates.

The temperature used for staining was incorrect

For Pentamers, try comparing staining at 22ºC (room temperature), to staining at 4ºC.  We do not recommend staining at 37ºC since this can yield considerable non-specific staining.

Incubation time with Pentamer was too long

Pentamer staining for 10 minutes at room temperature (22ºC) is sufficient. However, if staining at 4ºC the incubation time may be increased to 30 minutes. Incubation for longer periods may increase background.

Insufficient washing between staining steps

Cells should be washed with a 10x volume of buffer between staining steps (some specificities may require 2 washes between steps).

The stock Pentamer has not been stored according to instructions

Labeled Pentamers and Fluorotags should be stored consistently at 4ºC in the dark. Unlabeled and biotin-labeled Pentamers may also be stored at -80ºC.

B cells are interfering with the staining

Cells may be co-stained with anti-CD19 antibody to gate out B cells (see next section). Alternatively, anti-CD19 magnetic beads could be used to remove B cells prior to staining.

Buffer contains phenol red

If using RPMI-1640, HBSS or DMEM as a medium in which to stain cells it is recommended that this does not contain phenol red, which can contribute to autofluorescence and thus appear as non-specific staining on analysis plots.

Pentamer binds non-specifically to the cells

If cells in the sample are in a sub-optimal condition the Pentamer may bind non-specifically to the cell surface. This can be eliminated by first blocking the cells with 4 µg/ml pure IgG or 10% human or mouse serum. The Pentamer can then be added directly onto the sample + blocking reagent.

Common reasons for lack of staining

The antigen-specific population is not present

In addition to staining by flow cytometry, it is advisable to use an alternate method to verify the presence or absence of an antigen-specific population. Functional assays such as the study of cytokine secretion using ELISPOT, intracellular cytokine staining or a cytokine secretion assay are recommended.

Using an incorrect MHC Pentamer for the cell type/species

Check that your samples are positive for the MHC allele / tissue type of the MHC Pentamer you are intending to use and that the antigen you intend to investigate is only presented through this MHC allele.

Too little Pentamer for the number of cells

One test of Pentamer should stain 1-2 x 10⁶ antigen-specific cells. However, it is recommended that the Pentamer is titrated prior to use. Carry out a range of doubling dilutions from 1 test per 1 x 10⁶ cells down to 1/16 test per 1 x 10⁶ cells.

The antigen-specific population is below the threshold of detection

The threshold of detection of antigen-specific events depends on the type of cells used and their method of preparation. For human PBMCs the threshold is typically around 0.02%. Detecting a smaller population is possible but full protocol optimization may be required. An improvement in results may be achieved by enriching the population of T cells. This may be done using magnetic beads or by stimulation of cells in culture using peptides or antibodies.

Insufficient events acquired

When looking at rare populations, such as antigen-specific T cells, it is important to collect as many cells as possible; if expecting a result of only 0.1%, a sample size of 500,000 cells would show 500 dots on the plot. It is important to bear in mind the expected frequency of events to be collected and adjust the starting sample size accordingly.

Use of sub-optimal anti-CD8 antibody clone

The anti-CD8 antibody used for co-staining should be selected carefully as some clones interfere with Pentamer binding to the TCR. ProImmune has carried out extensive testing of Pentamers with different anti-CD8 clones and staining conditions. Clones LT8 (human) and KT15 (mouse) are recommended as they do not block binding of Pentamers to the TCR. Both of these antibody clones are available from ProImmune.

Reagent has expired

ProImmune guarantees all Pro5® MHC Pentamers for 6 months from delivery when stored according to instructions. All ProVE® MHC Pentamers are guaranteed for 3 months from delivery when stored according to instructions. From our regular stability testing we have determined that Pro5® and ProVE® MHC Pentamers are stable for longer than the indicated guarantee period. However, MHC Pentamers, like any other protein based reagent, will lose their activity eventually. Unlabeled and biotin-labeled Pentamers may be stored for longer periods at -80ºC.