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Submit a Bee Sample

bee geolocate2
  • Click to get your current geolocation. 
  • Complete submission form below. 
  • Please provide the address (or closest cross streets or copy & paste latitude/longitude) where bee was collected.
  • Drop-off or mail bee specimen(s) to:
Attn: 16-and-Bee
787 Allegheny Ave,
Costa Mesa, CA 92626 

 

 
 

Sample Submission Form

 
1000 characters left
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A blog on the latest bee news ... coming soon

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How is genetic testing of honeybee samples performed ?

 
Genetic markers that are characteristic of different honeybee subspecies/races can be analyzed by sensitive polymerase chain reaction (PCR) style tests.
 
PCR Test WorkflowOne such marker is the mitochondrial cytochrome b gene that carries a single nucoletide polymorphism (SNP) that distingushed between matrilineal African (Apis. m. scutellata) origin and various European races (Apis m. melifera and others).

AHB Mitotype
 
Bee specimens are dissected and a single leg is used for preparing a DNA sample. The leg is transferred to a microfuge tube and DNA extraction buffer added. The extraction buffer contains detergent solution to break open the cells and proteinase K which is a powerful protease enzyme able to digest the cells' proteins. This combination helps release the DNA.
 
A small amount of this starting honeybee DNA is then transferred to a PCR assay plate and mixed with a cocktail of different components. These incude:
 
  • Bee DNA (starting template)
  • dNTPs (the basic nucleotide building blocks of DNA)
  • DNA Forward/Reverse Primers (short oligonucleotide DNA fragments specific to the DNA region to be amplifed)
  • TaqMan Primer-dyes (sequence specific oligonculeotide primers coupled to different colored dyes to quantitate the different gene products of interest)
  • Buffer (to provide the correct salt and pH conditions)
  • Taq DNA polymerse (DNA copying enzyme)
PCR Principle
 
To amplify specific regions of the genome that contain diagnostic differences in the genetic code (e.g. mitochondrial cytochrome b gene), sequence specific DNA primers (short pieces of DNA that bind upstream and downstream of the target region), nucleotides (the basic building blocks of DNA) and a DNA copying enzyme (Taq DNA polymerase) are mixed together. The reactions are then run on a programmable thermal cycler PCR instrument as follows:
 
  1. Melting step: The PCR reaction starts by heating the sample to 95 oC. At this temperature the double stranded DNA helix separates (melts) to give two single strands.
  2. Annealing step: The reaction temperature is then lowered to 55 oC until the short forward/reverse DNA primers can bind (anneal) to their sequence specific regions.
  3. Elongation step: The temperature is then raised to 72 oC which is the optimal temperature for the Taq DNA polymerase to copy the DNA (elongation step). At this point every starting piece of target DNA has been copied to double the amount of product DNA.
  4. Quantitation step: The instrument will measure the amount of product present based on the fluorescence light signal produced by  primer-dye probes (TaqMan probes) that target the single nucleotide polymorphisms (SNP) present in the product. As the amount of product increases with each cycle, the fluorescence signal stengthens.
  5. Repeat cycle (steps 1-4): These three steps are then repeated another 40-times. With each cycle the amount of product doubles. After 40 cycles there could be millions of copies of product DNA produced from a single copy of starting template DNA.

A graph of the amount of DNA product (fluorescence intensity) versus the cycle # shows if there is a positive signal for amplification of the gene region of interest.

PCR Summary Plot

For the cytochrome b test, AHB DNA is detected by a TaqMan primer probe coupled to FAM dye (orange) whilst European bee DNA is detected by a probe couple to Hex dye (blue). In any sample these signals should be mutally exclusive hence giving a definitive result about the genetic heritage of the matrilineal (queen) line.

A positive result for the AHB SNP implies the bees are descendants of one of the 26 Apis m. scutellata queens that were accidently released in Brazil in 1956 and subsequently spread north throughout the Americas into the southern United States.

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Your Geolocation

 
Coming soon ... a geolocation app to provide your current longitude and lattitude when collecting bee samples.

 

How to Submit a Bee Sample for Genetic Testing
To contribute bee specimens for genetic analysis, please:
 
1) Collect 1 worker bee or drone per colony and place in a sample tube or Ziploc bag.
Label with <date-your initials-sample #> e.g. 01/16/24-AG-1
 
Collection of recently dead bees is acceptable, although live specimens are preferred to reduce DNA degradation. Place live specimens in freezer for 30 minutes prior to shipping.
 
2) Complete the webform below or download/printout the Sample Submission Form PDF.
 
Important: Please include location information (street address or cross-streets) where bee was collected.
This information is needed for accurate geospatial mapping of the results.
 
3) Drop off or send samples within 1-2 days to:
Re: 16-and-Bee
787 Allegheny Ave
Costa Mesa, CA 92626
 
4) Results can be found in the Data table and OC Bee Map.
 
 
Bee Sample Submission Form
 
1000 characters left

 

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