Nötrofil İzolasyon Protokolü

Neutrophil isolation protocol. This procedure will extract white blood cells from a whole blood sample equipment centrifuge and vials. Vortex sir needle and syringe syringe filter.

Milli pour brand MX gv 0.22 Micrometer materials. Hank spell and salt solution neutrophil separation requires two kinds of HBSS solutions. HBSS with calcium chloride will be used to make a solution with human serum albumin.

HBSS without calcium chloride will be used to suspend and wash the neutrophils. Please take special care to use the appropriate HBSS solution in this procedure. Human serum albumin or HSA is a protein in the blood plasma that maintains pH and SMO pressure.

Do not use bovine serum amalgamate red cell lysis buffer. This is manufactured by Roche Diagnostics, neutrophil Isolation Media NIM Cedar Line Labs Lymph light Poly separation media protected from light and kept in refrigerator for best results. All reagents should be at room temperature at time of use.

Remove reagents from refrigerator one hour before experiment. Prepare H-B-S-S-H-S-A solution for neutrophil separation. Pipette HBSS with calcium chloride into vial.

Draw HSA into syringe. Avoid trapping air bubbles. Remove the syringe needle and replace it with the filter.

Inject HSA through filter into HBSS vial vortex two mix when you have your other materials ready and at room temperature, acquire about 15 milliliters of whole blood. This will yield 10 to 15 milliliters of 10 to the eighth neutrophils. The donor should not have consumed alcohol or over the counter drugs for 24 hours prior to donating the blood sample.

These can disrupt the separation process. Whole blood may be anticoagulated with EDTA citrate or heparin by adding nine parts blood to one part K three EDTA sodium citrate, or heparin following manufacturer's instructions. The following steps will be described in this procedure.

Separate and remove plasma and monocytes. Separate and acquire a neutrophil layer lysing red blood cells free suspend neutrophils first separation. Acquire neutrophils in NIM layer.

Collect five milliliters of isolation media in centrifuge tube. Placing the isolation media lower in the tube allows it to act as a filter, as the centrifuge will force the blood down through it Carefully. Layer five milliliters of blood over the NIM for clean separation.

Be very careful to avoid mixing the solutions. Perform this step slowly and carefully and with your pipette tip close to the surface of the resolving media to prevent mixing centrifuge. The solution at 500 RCF for 35 minutes.

At 20 to 25 degrees Celsius, the blood should separate out into six distinct bands. The six bands are plasma monocytes, isolation media, neutrophils, more isolation media, and the red blood cell pellet at the bottom. If these six bands are not clear and distinct, the separation process was not clean and would need to be repeated.

Common causes of bad separation include old isolation media donor having consumed alcohol in the past 72 hours or donor having consumed other medicine such as Tylenol or aspirin. Carefully remove and discard the plasma monocytes and isolation media. Place these layers in a sealable tube and discard carefully pipette the layer of neutrophils and all of the isolation media beneath the neutrophils into a clean centrifuge file to recover as many neutrophils as possible.

It's often easiest to include some of the isolation media from the layer below as well. Do not disturb the pallet at the bottom. Second declaration, refine neutrophil layer.

Dilute the neutrophil solution to 10 milliliters with HBSS without calcium. Invert the tube a few times to suspend the cells centrifuge. The neutrophil solution.

350 RCF for 10 minutes. At 20 to 25 degrees Celsius, a red pellet should be present on the bottom of the tube containing neutrophils and residual red blood cells. Remove the supra natin with the pipette.

Be careful. to disturb the pellet at the bottom. Lysing the red blood cells.

The red blood cells in the sample must now be destroyed by lysis. To lys the residual red blood cells, add two milliliters of red cell lysis buffer to the tube to resus. Suspend the pellet vortex the vial at a setting of three to four.

Avoid increasing the vortex setting above four since this may cause the neutrophils to activate. It may be necessary to vortex for several seconds or to pulse the vortex to dissolve the palate. Centrifuge the lysis solution at 250 RCF for five minutes.

Use the soft start option to minimize damage to the sample. Remove the supra natin with pipette. Repeat the lysing process.

If require, release suspension of neutrophils, add 500 microliters HBSS without calcium to each tube. Vortex the pellet at a setting of three to four, dilute to 10 milliliters with HPSS without calcium centrifuge. The neutrophils at 250 RCF for five minutes aspirate the snat and discard.

Re suspend the pellet in 250 microliters of HBSS with HSA solution, two times 10 to the six. Neutrophils per milliliter are typically collected.