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Hawler Medical University
College of Health Sciences
Clinical Biochemistry Dept.
Ass. Lec. Amer Ali Khaleel
(M.Sc. Clinical Immunology)
Lab.2 : Whole Blood, Serum
& Plasma Collections
Practical Immunology and Serology
Copyright © 2016
Preparation and Separation of
Plasma:
The blood is transferred from a person’s vein to a test
tube and prevented from clotting (tube containing
anticoagulant e.g. Heparin, EDTA, Sodium Citrate,
Oxalate, Sodium Fluoride, Sodium Iodoacetate ) , this
preparation should be mixed immediately and
thoroughly to avoid clotting, and centrifuged at 2500-
3000 rpm for 5-10 min.
Preparation and Separation of
Plasma:
It separates into two layers. The upper liquid layer,
called plasma, represents about 55% of the volume
of whole blood. The lower layer consists of red blood
cells (erythrocytes), white blood cells (leukocytes),
and blood platelets (thrombocytes). Collectively,
these are called the formed (cellular) elements and
represent about 45% of the volume of whole blood.
Preparation and Separation of
Serum:
• If blood is transferred from a person’s vein to a test tube
without containing anticoagulant and then allowed the
blood to clot at room temperature for 15 to 30 minutes,
when the blood has clotted completely and then
centrifuged at 2500-3000 rpm for 5-10 min. it separates into
two layers, the upper liquid layer called serum and the
lower layer consists of formed elements.
• Serum =Plasma- Fibrinogen(coagulant factor)
Laboratory Specimens:
Most Common
•Blood samples
•Urine samples
Swabs
•Vaginal swabs
•Wound swabs
•Nose swabs
•Pernasal swabs
•Ear swabs
•Eye swabs
•Throat swabs
Additional
•Biopsy material
•Cerebrospinal fluid
•Stool samples
•Fungal samples of hair, nail and skin
•Naso-pharyngeal aspirate
•Sputum
•Semen
•Vaginal secretion
•Saliva
•Tears
•Cerumen (earwax)
•Sweat
Body Fluid
•Percardial fluid
•Pleural fluid
•Synovial fluid
•Vitreous humour
•Amniotc fluid
Important note:
• The color of the serum and plasma must be clear yellow
and there is no any turbidity (cloudy) or if any white color
it shows the high proportion of fat in it which affects the
result of the analysis.
• Similarly, if the color is reddish, it indicates the breaking of
red blood cells, which affects a significant impact on some
of the results.
Which is more appropriate Plasma or Serum
or whole blood for doing blood biochemical
estimations?
• It depends on type of analyte to be determined.
• You better use serum rather than plasma.
Anticoagulate in the plasma interferes with many
biochemical parameters particularly trace
elements as lead and mercury are bond
preferably on erythrocytes, therefore for its
determination, the whole blood is preferred.
Method for Serum Preservation
(Storage):
• In normal condition and the right is that the samples are direct do test
without delay but, if necessary keeping the sample must be following
in mind:
• Must separated sample and stored at low temperature in the
refrigerator or freezer.
• Never preserves whole blood samples such as complete blood count
in the freezer.
• Some samples have special conditions, such as the conservation
Bilirubin must be kept in the dark.
• There are samples should never delay ,such as analysis of
prothrombin and erythrocyte sedimentation analysis .
Method for Serum Preservation
(Storage):
1. Preservation for short time,freezing method is followed between
(-4 to -28°C).
2. Preservation for Long time, freezing method is (-86°C).
Benchtop FreezerUpright Freezer
Notes:
• How long can frozen human serum be stored?
Frozen blood can be stored for 10 years from the date of
blood collection.
• It is important to avoid freeze-thaw cycles because this is
detrimental to many serum components.
• The serum put in polypropylene microcentrifuge tube.
Common Serum or Plasma Preparation
Errors:
1-Failure to separate serum or plasma from red cells within 30 to 45
minutes of venipuncture.
2-Hemolysis (occurs when the membrane surrounding red blood cells
is disrupted and hemoglobin and other intracellular components
escape into the serum or plasma. Hemolyzed serum or plasma varies in
color from faint pink to bright red, rather than the normal straw color.
Grossly or moderately hemolyzed specimens may be rejected and even
slight hemolysis may alter certain test results).
How To Prevent Hemolysis:
1. Do not leave tourniquet for longer than one minute.
2. Allow alcohol to dry completely before puncturing the
skin.
3. Use a properly sized needle for routine collections.
4. Do not remove the needle from the vein with the vacuum
tube still engaged.
5. Make sure sample is not exposed to extreme heat or cold.
6. Allow blood to clot completely prior to centrifugation.
7. Avoid vigorous mixing or shaking of tubes.
8. Do not centrifuge specimens at higher speed or for longer
than necessary.
Differences between in vitro, in vivo, and in
silico studies
There are three broad categories of experiments:
In vitro (Latin for within the glass) refers to the technique of performing
a given procedure in a controlled environment outside of a living
organism.
In vivo (Latin for “within the living”) refers to experimentation using a
whole, living organism as opposed to a partial or dead organism.
In silico is an expression used to mean “performed on computer or via
computer simulation.
Serological
Reactions:
• Antigen-antibody reaction (binding) in vitro are known as
serological reactions, its useful for detection and
measurement either antibody (Ab) or antigen (Ag) in the
serum.
Uses:
1- Diagnosis of infections.
2- Evaluation of the immunological status.
• Antigens (Ag) : Are molecules (substances) recognised by
the immune system, which induce an immune response
examples bacteria, viruses, parasites & fungi.
• Antibodies (Immunoglobulin): Are proteins produced by
plasma cells in response to stimulation of B cell by foreign
antigen, basic structure of immunoglobulin is Y shaped
structure, there are five immunoglobulin classes of antibody
molecules found in serum: IgG, IgM, IgA, IgE and IgD.
Some Concept:
Serological Techniques and Immune
Assays:
•Numerous types of serologic test differ in their speed and
sensitivity, so the most effective test have high specificity and
sensitivity, some are strictly qualitative (positive or negative)
and others are quantitative (amount measured).
Serological Techniques and Immune
Assays:
There are several different methods used in serological tests:
1.Agglutination test.
2.Precipitation test.
3.Labeled Immune assay (immunoassay).
A.Radioimmunoassay (RIA).
B.Fluorescent immunoassay (FIA).
C.ElectroChemiluminescent immunoassays (ECL).
D.Enzyme immunoassay (EIA) & Enzyme linked immunosorbent assay
(ELISA).
Principle of Serological Tests:
• A reaction between antigen (Ag) and antibody
(Ab) to produce a DETECTABLE reaction.
• Antigen-antibody reaction are visible by clumps,
precipitates, color changes, emitting photons &
release of radioactivity.
Agglutination Reaction
(test):
• The interaction (immune reaction) between antibody and a
particulate antigen resulting a visible clumping called
agglutination. Antibodies that produce such reactions are
called agglutinins while antigens are called agglutinogen.
• Agglutination: This reaction done between Ab & insoluble
Ag is part of the surface of some particulate material (such
as Erythrocytes, Bacterial cells, Inert carriers such as
polystyrene latex particles).
• Purpose: Agglutination reactions used to detect either the
presence of antigen or antibody in a sample.
Figure: Phases of agglutination. (Stevens, 2010) A) Sensitization, physical
attachment of Ag & Ab. B) Network formation.
Clinical Applications of agglutination test:
(Reagents)
• ANA (Antinuclear antibody) test for diagnosis nuclear autoantibodies.
• ASO (Antistreptolysin O) test for diagnosis of Streptococcus bacteria.
• Brucella agglutination test for diagnosis of brucellosis.
• CRP (C-Reactive Protein) to check for inflammation in the body.
• IM (Infectious Mononucleosis) or Monospot screening test for infections
mononucleosis.
• Latex test for rheumatoid factor.
• PT (Pregnancy testing) for detection Beta-HCG.
• RF (Rheumatoid factor test) detects autoantibodies present in Rheumatoid
arthritis.
• TPHP (Treponema pallidum particle agglutination assay) screening test for syphilis.
• VDRL (Venereal Disease Research Laboratory test) screening test for syphilis.
• Widal test for diagnosis of salmonellosis.
1-Prepartion of serum.
2-Prepartion of plasma.
3-Preservation methods.
Practical Part
Whole blood, serum & plasma collections

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Whole blood, serum & plasma collections

  • 1. Hawler Medical University College of Health Sciences Clinical Biochemistry Dept. Ass. Lec. Amer Ali Khaleel (M.Sc. Clinical Immunology) Lab.2 : Whole Blood, Serum & Plasma Collections Practical Immunology and Serology Copyright © 2016
  • 2. Preparation and Separation of Plasma: The blood is transferred from a person’s vein to a test tube and prevented from clotting (tube containing anticoagulant e.g. Heparin, EDTA, Sodium Citrate, Oxalate, Sodium Fluoride, Sodium Iodoacetate ) , this preparation should be mixed immediately and thoroughly to avoid clotting, and centrifuged at 2500- 3000 rpm for 5-10 min.
  • 3. Preparation and Separation of Plasma: It separates into two layers. The upper liquid layer, called plasma, represents about 55% of the volume of whole blood. The lower layer consists of red blood cells (erythrocytes), white blood cells (leukocytes), and blood platelets (thrombocytes). Collectively, these are called the formed (cellular) elements and represent about 45% of the volume of whole blood.
  • 4. Preparation and Separation of Serum: • If blood is transferred from a person’s vein to a test tube without containing anticoagulant and then allowed the blood to clot at room temperature for 15 to 30 minutes, when the blood has clotted completely and then centrifuged at 2500-3000 rpm for 5-10 min. it separates into two layers, the upper liquid layer called serum and the lower layer consists of formed elements. • Serum =Plasma- Fibrinogen(coagulant factor)
  • 5.
  • 6. Laboratory Specimens: Most Common •Blood samples •Urine samples Swabs •Vaginal swabs •Wound swabs •Nose swabs •Pernasal swabs •Ear swabs •Eye swabs •Throat swabs Additional •Biopsy material •Cerebrospinal fluid •Stool samples •Fungal samples of hair, nail and skin •Naso-pharyngeal aspirate •Sputum •Semen •Vaginal secretion •Saliva •Tears •Cerumen (earwax) •Sweat Body Fluid •Percardial fluid •Pleural fluid •Synovial fluid •Vitreous humour •Amniotc fluid
  • 7. Important note: • The color of the serum and plasma must be clear yellow and there is no any turbidity (cloudy) or if any white color it shows the high proportion of fat in it which affects the result of the analysis. • Similarly, if the color is reddish, it indicates the breaking of red blood cells, which affects a significant impact on some of the results.
  • 8. Which is more appropriate Plasma or Serum or whole blood for doing blood biochemical estimations? • It depends on type of analyte to be determined. • You better use serum rather than plasma. Anticoagulate in the plasma interferes with many biochemical parameters particularly trace elements as lead and mercury are bond preferably on erythrocytes, therefore for its determination, the whole blood is preferred.
  • 9. Method for Serum Preservation (Storage): • In normal condition and the right is that the samples are direct do test without delay but, if necessary keeping the sample must be following in mind: • Must separated sample and stored at low temperature in the refrigerator or freezer. • Never preserves whole blood samples such as complete blood count in the freezer. • Some samples have special conditions, such as the conservation Bilirubin must be kept in the dark. • There are samples should never delay ,such as analysis of prothrombin and erythrocyte sedimentation analysis .
  • 10. Method for Serum Preservation (Storage): 1. Preservation for short time,freezing method is followed between (-4 to -28°C). 2. Preservation for Long time, freezing method is (-86°C). Benchtop FreezerUpright Freezer
  • 11. Notes: • How long can frozen human serum be stored? Frozen blood can be stored for 10 years from the date of blood collection. • It is important to avoid freeze-thaw cycles because this is detrimental to many serum components. • The serum put in polypropylene microcentrifuge tube.
  • 12. Common Serum or Plasma Preparation Errors: 1-Failure to separate serum or plasma from red cells within 30 to 45 minutes of venipuncture. 2-Hemolysis (occurs when the membrane surrounding red blood cells is disrupted and hemoglobin and other intracellular components escape into the serum or plasma. Hemolyzed serum or plasma varies in color from faint pink to bright red, rather than the normal straw color. Grossly or moderately hemolyzed specimens may be rejected and even slight hemolysis may alter certain test results).
  • 13. How To Prevent Hemolysis: 1. Do not leave tourniquet for longer than one minute. 2. Allow alcohol to dry completely before puncturing the skin. 3. Use a properly sized needle for routine collections. 4. Do not remove the needle from the vein with the vacuum tube still engaged. 5. Make sure sample is not exposed to extreme heat or cold. 6. Allow blood to clot completely prior to centrifugation. 7. Avoid vigorous mixing or shaking of tubes. 8. Do not centrifuge specimens at higher speed or for longer than necessary.
  • 14. Differences between in vitro, in vivo, and in silico studies There are three broad categories of experiments: In vitro (Latin for within the glass) refers to the technique of performing a given procedure in a controlled environment outside of a living organism. In vivo (Latin for “within the living”) refers to experimentation using a whole, living organism as opposed to a partial or dead organism. In silico is an expression used to mean “performed on computer or via computer simulation.
  • 15. Serological Reactions: • Antigen-antibody reaction (binding) in vitro are known as serological reactions, its useful for detection and measurement either antibody (Ab) or antigen (Ag) in the serum. Uses: 1- Diagnosis of infections. 2- Evaluation of the immunological status.
  • 16. • Antigens (Ag) : Are molecules (substances) recognised by the immune system, which induce an immune response examples bacteria, viruses, parasites & fungi. • Antibodies (Immunoglobulin): Are proteins produced by plasma cells in response to stimulation of B cell by foreign antigen, basic structure of immunoglobulin is Y shaped structure, there are five immunoglobulin classes of antibody molecules found in serum: IgG, IgM, IgA, IgE and IgD. Some Concept:
  • 17. Serological Techniques and Immune Assays: •Numerous types of serologic test differ in their speed and sensitivity, so the most effective test have high specificity and sensitivity, some are strictly qualitative (positive or negative) and others are quantitative (amount measured).
  • 18. Serological Techniques and Immune Assays: There are several different methods used in serological tests: 1.Agglutination test. 2.Precipitation test. 3.Labeled Immune assay (immunoassay). A.Radioimmunoassay (RIA). B.Fluorescent immunoassay (FIA). C.ElectroChemiluminescent immunoassays (ECL). D.Enzyme immunoassay (EIA) & Enzyme linked immunosorbent assay (ELISA).
  • 19. Principle of Serological Tests: • A reaction between antigen (Ag) and antibody (Ab) to produce a DETECTABLE reaction. • Antigen-antibody reaction are visible by clumps, precipitates, color changes, emitting photons & release of radioactivity.
  • 20. Agglutination Reaction (test): • The interaction (immune reaction) between antibody and a particulate antigen resulting a visible clumping called agglutination. Antibodies that produce such reactions are called agglutinins while antigens are called agglutinogen. • Agglutination: This reaction done between Ab & insoluble Ag is part of the surface of some particulate material (such as Erythrocytes, Bacterial cells, Inert carriers such as polystyrene latex particles). • Purpose: Agglutination reactions used to detect either the presence of antigen or antibody in a sample.
  • 21. Figure: Phases of agglutination. (Stevens, 2010) A) Sensitization, physical attachment of Ag & Ab. B) Network formation.
  • 22. Clinical Applications of agglutination test: (Reagents) • ANA (Antinuclear antibody) test for diagnosis nuclear autoantibodies. • ASO (Antistreptolysin O) test for diagnosis of Streptococcus bacteria. • Brucella agglutination test for diagnosis of brucellosis. • CRP (C-Reactive Protein) to check for inflammation in the body. • IM (Infectious Mononucleosis) or Monospot screening test for infections mononucleosis. • Latex test for rheumatoid factor. • PT (Pregnancy testing) for detection Beta-HCG. • RF (Rheumatoid factor test) detects autoantibodies present in Rheumatoid arthritis. • TPHP (Treponema pallidum particle agglutination assay) screening test for syphilis. • VDRL (Venereal Disease Research Laboratory test) screening test for syphilis. • Widal test for diagnosis of salmonellosis.
  • 23. 1-Prepartion of serum. 2-Prepartion of plasma. 3-Preservation methods. Practical Part

Editor's Notes

  1. WHAR ARE YOU DO I
  2. Fahrenheit to Celsius (ºF to ºC) http://www.metric-conversions.org/temperature/fahrenheit-to-celsius.htm WHY Bilirubins are usually in tubes and kept in dark tubes and out of the light? Because bilirubin break done by light
  3. Fahrenheit to Celsius (ºF to ºC) http://www.metric-conversions.org/temperature/fahrenheit-to-celsius.htm fridge
  4. WHAT ARE DOING IF YOUR SAMPLE IS HEMLOYSIS?
  5. The use of laboratory animals (mice, guinea pigs, rabbits) is now limited due to the advancement in medical microbiological techniques. In silico techniques are developed particularly as an alternative to animal experimentation.
  6. Agglutination test. (8 types) Precipitation test. (7 types)
  7. Blood group and type (ABO and Rh). (Hematology Department) Coombs test. (Hematology Department) Cross-match (Hematology Department)