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  5. SAS-MX Acid HB-10
  6. Instrucciones de uso

helena BioSciences SAS-MX Acid HB-10 Instrucciones De Uso página 5

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S S A A M M P P L L E E C C O O L L L L E E C C T T I I O O N N A A N N D D P P R R E E P P A A R R A A T T I I O O N N
Freshly collected EDTA or heparin anticoagulated blood is the specimen of choice. Samples can be
stored refrigerated at 2...6°C for up to 1 week. For optimal results, saline washed red cells should be
used to prepare lysates. This removes possible interference from plasma proteins.
a) Mix 200µL of well mixed whole blood with 1000µL of saline solution.
b) Centrifuge to sediment the red cells.
c) Remove 1000µL of the supernatant and discard.
d) Add a further 1000µL of saline solution and mix well.
e) Repeat steps b-d x2.
f)
Following the final centrifugation, remove 1000µL of supernatant and treat the remaining sample
as whole blood, or remove all of the supernatant and treat the remaining sample as washed packed
cells.
Dilute each patient sample / control to a haemoglobin concentration of 0.5-1.5 g/dL with Haemoglobin
Lysing Agent.
S S T T E E P P - - B B Y Y - - S S T T E E P P P P R R O O C C E E D D U U R R E E
1. Remove the gel from the packaging and place on a paper towel. Blot the gel surface with a blotter
C, discard the blotter.
2. Align the sample application template with the arrows at the edge of the gel. Place a blotter A on
top of the template and rub a finger across the slits to ensure good contact. Remove the blotter
and retain for use in Step 5.
3. Apply 3µl of sample to each slit and allow to absorb for 5 minutes.
4. Whilst the samples are absorbing, pour 30ml of buffer into each inner section of the SAS-MX
Chamber.
5. Following sample absorption, blot the template with the blotter A retained from Step 2 and
remove the blotter and template.
6. Position the gel in the chamber agarose side down, aligning the positive (+) and negative (-) sides
with the corresponding positions in the chamber.
7. Electrophorese the gel: 50 volts, 30 minutes
8. Following electrophoresis, immerse the gel in fixative / destain solution for 5 minutes.
9. Immerse the gel in stain solution for 15 minutes.
10. Rinse the gel briefly in fixative / destain solution to remove excess stain, and dry in a drying oven
with forced air at 60...70°C.
11. Destain the gel in 2 x 2 minute washes of fixative / destain solution or until the background is clear.
12. Wash the gel briefly in purified water and dry.
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SAS-MX ACID HB-10
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