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Frequently
Asked Questions - ELISA
Frequently Asked Questions - INDOORŪ Allergen Analysis
Service
Solutions
and reagents for ELISA assays
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Frequently Asked Questions - ELISA Sensitivity
and reproducibiltity of ELISA for indoor allergens Q1 What is the difference between the Der p 1 ELISA kits, EL-DP1 and EL-DP1A? A
INDOOR Biotechnologies markets two ELISA kits to measure Der p 1 which
differ in the combination of monoclonal antibodies that are used in the
assays: Q2 We noticed that the assay was very slow in developing (and never reached OD 2.0). Is this a problem? A There is definitely a problem with your results - the control curves should read OD 2.0-2.4 at the highest concentration and have sensitivity down to 1-4ng/ml. If not reaching an OD of 2.0 is the case with all your assays, it suggests that it may have something to do with the substrate system and color development. A Have the biotinylated reagents been frozen at any time during storage? This may reduce the sensitivity of those mAbs. A Are you making up the reagents or using buffer tablets? We have found that some buffer tablets do not work as well as fresh made solutions. We usually keep all solutions for less than a month at 4°C without Thimerosal. A Has sodium azide been used in any of the reagents as preservatives? This would stop the color development since it is an inhibitor of horseradish peroxidase. A When making up Solution B for the ABTS is the correct form of Sodium Phosphate used? The sodium phosphate has to be Dibasic, Heptahydrate (Na2HPO4·7H20). A Are you adding enough hydrogen peroxide to the ABTS solution? Use 1µl of 30% H2O2/ml of ABTS solution. A Has the streptavidin-peroxidase been diluted correctly? A Is the pH of the ABTS citrate buffer correct? The pH of the ABTS solution should be pH 4.2 and should be close to that pH before adjustment. If it is far off, solution A or B or their proportions are probably incorrect. Q3 The backgrounds for our assays have been high. What could be the cause of this? A The background on the assay is usually higher in assays where the secondary antibody is a rabbit polyclonal. The background is usually around 0.15 OD. Other causes of the high background may be: A
The source of the peroxidase labeled Goat anti Rabbit IgG antibody.
We use material from BioSource International and also Jackson Laboratories.
Both work well with very low backgrounds. A How long is the ABTS substrate kept at 4°C? It is usually stable for about one month in the fridge. It can start to turn green and give high backgrounds if kept for longer periods. The ABTS solution should be more or less colorless for use in the assay. The same goes for the other solutions. We usually keep all solutions for less than a month at 4°C without Thimerosal. A Block the plates for 30 minutes with 1%BSA/PBS-T before adding allergen solutions. Q4 Can we keep antibody-coated micro-wells in storage? How long can they be stored and at what conditions? A The coated plates can only be stored for a short period e.g. over the weekend or up to a week. We usually leave plates coated with antibody solution and wrapped in plastic film in the lab fridge or cold room. We have not tried longer storage times. Q5 Can we substitute the ABTS with OPD or TMB? We had difficulties keeping the ABTS under the conditions required by Sigma (in a desiccator, under Argon). A You can use OPD or TMB. We do not keep ABTS under Argon (it doesn’t appear to be necessary). We have good results with ABTS. Q6 Should the dust samples be stored at 4°C or should they be frozen? A We routinely keep house dust samples at 4°C prior to assay, but once extracted they should be stored at -20°C. Q7 How can I stop the enzyme reaction in the ELISA? A The reaction can be stopped by adding 0.1ml 0.002M sodium azide to each well. Most ELISA readers scan plates in 5-20 seconds and plates can be read once the OD reaches 2.0-2.4 without stopping the reaction. Azide can be added if a large number (5-10 plates) are set up, or if the plates need to be preserved for any other reason e.g. taking photographs. Q8 What temperature is used for the ELISA incubations? A Coating the ELISA plates with the capture mAb is carried out overnight at 4°C. All other steps are carried out at room temperature, usually 20-25°C.Q9
I would like Indoor Biotechnologies to check the allergen
content of my allergen extracts or solutions. What quantity should I send? Q10
Could you please tell me how many dust (or air) samples can we analyse
with one ELISA kit? How many do you recommend? If a control curve is included in duplicate on every plate, with 4 control (PBS-T) wells, it will use 24 microtiter wells, leaving 72 wells for samples. Typically, we use 4 doubling dilutions for each dust sample (1/10, 1/20, 1/40, 1/80 for mite allergens), which means that 18 samples can be tested on a plate. Under these conditions, one 20 plate ELISA kit could be used to analyse 18 x 20 = 360 samples. However, the plate to plate variation for most assays is less than 10% and we normally do not need to have a control curve on every plate. For example, we might set up four plates with only one control curve. Under these conditions, 24 samples can be analysed per plate, together with 18 on the same plate as the control curve, or 90 samples in all on 4 plates. This would mean 450 samples could be analysed using the 20 plate ELISA kit. We use four dilutions per sample so that we can in most cases obtain results on >90% of the samples in a single assay. The four dilutions increase the probability of having at least two points on the linear part of the control curve for each sample. It may be possible to use fewer dilutions, if the samples are known to have allergen levels in a particular range. Other samples, e.g. allergenic extracts, may have very high allergen levels and have to be assayed at doubling dilutions starting at 1/100 or 1/1000, and may need to be serially diluted across the ELISA plate. Air samples usually contain low levels of allergen and are assayed at 1/2, 1/4, 1/8, and 1/16 dilution. |
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Frequently
Asked Questions - INDOOR®
Allergen
Analysis Service Q10
I want to send some dust samples to Indoor Biotechnologies
for allergen analysis. How much dust do you need? A For the analysis lab to analyze for the allergen levels in bulk dust samples, we need 100mg of fine dust. Samples of bulk dust will not be processed if there is less than 30mg of fine dust. A For air sampling cassettes, the whole filter is extracted with 1ml of PBS extraction solution and the results are reported as ng or µg allergen per filter. Q11
I would like Indoor Biotechnologies to check the allergen
content of my allergen extracts or solutions. What quantity should I send? Q12 I am preparing dust samples for analysis in my laboratory. Do I need to sieve the dust? A Whether to sieve the dust or not is determined by the quality of the dust. We do not routinely sieve dust collected from beds and soft furnishings. Carpet samples are sieved (e.g. using a No.45 mesh screen, 355um diameter sieve) to separate the fiber and large particles from fine dust. We recommend the use of the MITEST dust collector which greatly reduces the need for sieving dust. After collecting a dust sample using the MITEST dust collector, remove the nylon filter containing the dust sample insert, invert the filter and tap the dust onto a piece of weigh paper. The fine dust falls before the fibers come out of the filter. Q13
How should dust samples and dust extracts be stored? A Dust samples prior to extraction should be stored in a dry place at room temperature. Dust extracts should be stored frozen in a -20C freezer. Q14
What are the procedures for sampling and submitting
samples for INDOOR Allergen Analysis Service? A Please see Collecting Dust Samples and Submitting Dust Samples. Q15
What method do you recommend for preparation of extracts? A Please see sample extraction procedures. |