Atlas of hematology practical and clinical diagnosis (thieme 2004) by Pili Gabriel

Atlas of hematology practical and clinical diagnosis (thieme 2004)

Procedures, Assays, and Normal Values

Taking Blood Samples Since cell counts are affected by the state of the blood circulation, the conditions under which samples are taken should be the same so far as possible if comparable values are desired.

This means that blood should always be drawn at about the same time of day and after at least eight hours of fasting, since both circadian rhythm and nutritional status can affect the findings. If strictly comparable values are required, there should also be half an hour of bed rest before the sample is drawn, but this is only practicable in a hospital setting. In other settings (i.e., outpatient clinics), bringing portable instruments to the relaxed, seated patient works well. A sample of capillary blood may be taken when there are no further tests that would require venous access for a larger sample volume. A wellperfused fingertip or an earlobe is ideal; in newborns or young infants, the heel is also a good site. If the circulation is poor, the blood flow can be increased by warming the extremity by immersing it in warm water. Without pressure, the puncture area is swabbed several times with 70% alcohol, and the skin is then punctured firmly but gently with a sterile disposable lancet. The first droplet of blood is discarded because it may be contaminated, and the ensuing blood is drawn into the pipette (see below). Care should be taken not to exert pressure on the tissue from which the blood is being drawn, because this too can change the cell composition of the sample. Obviously, if a venous blood sample is to be taken for the purposes of other tests, or if an intravenous injection is going to be performed, the blood sample for hematological analysis can be taken from the same site. To do this, the blood is allowed to flow via an intravenous needle into a specially prepared (commercially available) EDTA-treated tube. The tube is filled to the 1-ml mark and then carefully shaken several times. The very small amount of EDTA in the tube prevents the blood from clotting, but can itself be safely ignored in the quantitative analysis.