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Blood investigations in Dental Practice.Dr Ayesha

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Blood investigations

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Blood investigations in Dental Practice.Dr Ayesha

  1. 1. BLOOD INVESTIGATIONS IN DENTAL PRACTICE Presented by: Dr.Ayesha Taha JR I Department of Pedodontics and Preventive Dentistry SPPGIDMS, Lucknow
  2. 2. CONTENT INTRODUCTION HAEMOSTASIS SIGNIFICANCE OF BLOOD INVESTIGATION COLLECTION OF BLOOD SAMPLE TYPES OF HEMATOLOGICAL INVESTIGATIONS •Complete Blood Count •WBC count •Differential Leukocyte count •Hemoglobin •Hematocrit •Erythrocytes indices •Platelets •Bleeding time
  3. 3. •Capillary Fragility Test •Clotting Time •Erythrocyte Sedimentation Rate HEMATOLOGICAL INVESTIGATIONS (not so frequent in dentistry) •Prothrombin Time •Partial Thromboplastin Time •INR OTHER BLOOD TESTS DENTAL MANAGEMENT OF BLEEDING DISORDER CONCLUSION
  4. 4.  Various laboratory Investigations are sometimes required for diagnosis and treatment planning of disorder related to oral cavity.  These can detect abnormalities such as • Infection • Anaemia • Allergies  Blood is also examined for grouping and cross-matching INTRODUCTION
  5. 5. A NORMAL TEST result is just as significant as an abnormal result. A normal result does not mean that the test was unnecessary. When a result is normal, it not only helps to rule out diseases, but it also establishes a baseline for the clinician.
  6. 6. Either whole blood is used to count blood cells, or the blood cells are separated from the fluid that contains them. This fluid is called Plasma or Serum. • Blood to be separated for serum samples is collected in a plain clotting tube (containing beads treated with a clotting activator). •Blood NOT to be separated for serum samples is collected in a tube containing lithium heparin (or beads treated with lithium heparin).
  7. 7. 1. Vascular phase :Vasoconstriction, immediately 2. Platelet phase : Adhesion & aggregation,Platelet plug formation. 3. Coagulation phase : later, contains extrinsic & intrinsic pathways 4. Metabolic (fibrinolytic) phase: release antithrombotic agents. HAEMOSTASIS
  8. 8. SIGNIFICANCE OF BLOOD INVESTIGATION Blood investigation helps in diagnosing • Leukopenia • Thrombocytopenia • Myeloma • Anemia *Iron deficiency *Aplastic *Sickle cell anemia • Thalassemia • Acute and Chronic leukemia • liver disease • Myxedema •Diabetes
  9. 9. COLLECTION OF BLOOD SAMPLE •CAPILLARY BLOOD SPECIMENS: The specimen is obtained by pricking the patient`s finger . •VENOUS BLOOD SPECIMEN: Most Commonly used method. Venipuncture is usually performed in ANTECUBITAL vein.
  10. 10. •WBC count •Differential Leukocyte count •RBC count •Hemoglobin •Hematocrit •Erythrocytes indices •Platelet Count •Bleeding time •Capillary Fragility Test •Clotting Time •Erythrocyte Sedimentation Rate TYPES OF HEMATOLOGICAL INVESTIGATIONS Complete Blood Count
  11. 11. COMPLETE BLOOD COUNT Complete blood count (CBC) is one of the most commonly ordered blood tests. The complete blood count is the calculation of the cellular (formed elements) of blood.
  12. 12. What are the components of the complete blood count (CBC)? The complete blood count, or CBC, lists a number of many important values. Typically, it includes the following: • White blood cell count (WBC or leukocyte count) • WBC differential count WBC • Red blood cell count (RBC or erythrocyte count) • Hematocrit (Hct) • Hemoglobin (Hbg) • Mean corpuscular volume (MCV) • Mean corpuscular hemoglobin (MCH) • Mean corpuscular hemoglobin concentration (MCHC) RBC • Platelet countPLATELET
  13. 13. •White blood cell count (WBC) is the number of white blood cells in a volume of blood. •This can also be referred to as the Leukocyte Count •It can be expressed in international units = 4.3 to 10.8 x 109 cells per liter. • Normal range of WBC= 4,500 - 10,000 cells/mm3 of blood. •Number of cells are usually counted with the help of Neubauer’s counting chamber WBC/Leukocyte Count
  14. 14. A high white blood cell count usually indicates: 1. An increased production of white blood cells to fight an infection 2. A reaction to a drug that increases white blood cell production 3. A disease of bone marrow, causing abnormally high production of white blood cells 4. An immune system disorder that increases white blood cell production.
  15. 15. Specific causes of Leukocytosis: 1. Infection- Acute and Chronic 2. Leukaemia 3. Polycythemia 4. Trauma 5. Exercise , Stress and fear 6. After general anesthesia 7. Allergy 8. Drugs, such as corticosteroids and epinephrine 9. Rheumatoid arthritis 10. Smoking
  16. 16. Specific causes of Leukopenia: 1. Aplastic anaemia 2. Influenza, measles and Respiratory tract infection 3. Catarrhal Jaundice 4. Early Leukaemia 5. Depression of Bone marrow 6. Drug and chemical toxicity 7. Shock
  17. 17. WBC Granulocytes Neutrophils Eosinophils Basophils Agranulocytes Lymphocytes Monocytes White blood cell (WBC) differential count: White blood cells are comprised of several different types of cells that are differentiated, or distinguished, based on their size and shape. Differential Count WBC
  18. 18. Normal values: • Granulocytes (or polymorphonuclears) Neutrophils:2.0–7.0×109/l (40–80%) Eosinophils: 0.02–0.5×109/l (1–6%) Basophils: 0.02–0.1×109/l (< 1–2%) • Agranulocytes (or mononuclear) Lymphocytes: 1.0–3.0×109/l (20–40%) Monocytes: 0.2–1.0×109/l (2–10%)
  19. 19. CLINICAL SIGNIFICANCE Neutrophils INCREASES in: DECREASES in: Inflammatory disease Aplastic Anaemia Stress Cyclic Neutropenia Exercise Malignant Neutropenia Pregnancy Early Leukemia Infection Excitement Eosinophils INCEASES in: DECREASES in: Parasitic infections Immune defect Hypersensitivity/ Acute stress Allergic responses Typhoid Fever Scarlet Fever Aplastic Anaemia
  20. 20. Basophils INCREASES in: DECREASES in: Chronic leaukemia Acute Infection Myelofibrosis Severe injury Polycythemia Lymphocytes INCEASES in: DECREASES in: Lymphocytic Leukemia Aplastic Anaemia Mumps Whooping Cough Chronic Infection
  21. 21. •Monocytes INCREASES in: DECREASES in: Hodgkin disease Aplastic Anaemia Monocytic Anaemia Acute Leukemia Malaria – Kala Azar SABE TB
  22. 22. RBC Count •Red Blood cell count (RBC) signifies the number of red blood cells in a volume of blood. • Normal range : 4.2 to 5.9 million cells/cmm. • This can also be referred to as the Erythrocyte count • It can be expressed in international units:4.2 to 5.9 x 1012 cells per liter.
  23. 23. •An increase in red blood cell mass is known as Polycythemia. •Polycythemia Vera is a disease of unknown origin that results in an abnormal increase in red blood cells. •CAUSES: •Normal physiological increases in the RBC count occurs at high altitudes or after strenuous physical training. • Drugs: Gentamicin Methyldopa •Smokers also have a higher number of red blood cells than non- smokers. INCREASE in RBC Count
  24. 24. DECREASE in RBC Count •Massive RBC loss, such as acute hemorrhage • Abnormal destruction of red blood cells • Lack of substances needed for RBC production • Chemotherapy or radiation side effects from treatment of bone marrow malignancies such as leukemia can result in bone marrow suppression.
  25. 25. HEMOGLOBLIN Hemoglobin is the protein molecule within red blood cells that carries oxygen and gives blood its red color. •Normal range =13-18 grams per dl for men and 12-16 grams per dl for women •International units= 8.1 to 11.2 millimoles/L for men 7.4 to 9.9 milimoles/L for women
  26. 26. Increase in Hb *Benign neoplasm of brain and CNS *Carcinoma of the kidney * Cholera *Diarrhoea *Pheochromocytoma *Polycythemia vera Decrease in Hb *Aplastic anaemia *Anti-retroviral drugs for HIV infection Cirrhosis *Hodgkin's lymphoma *Hypothyroidism *Kidney disease *Lead poisoning *Leukaemia *Multiple myeloma *Vitamin deficiency anaemia
  27. 27. A low haemoglobin count can also be due to blood loss Diseases and conditions that cause the body to destroy red blood cells faster than they can be made: • Enlarged spleen (splenomegaly) • Sickle cell anemia • Thalassemia • Vasculitis
  28. 28. •It is a measure of volume percent of packed red blood cells to that of whole blood. •This is usually measured by spinning down a sample of blood in a test tube, which causes the red blood cells to pack at the bottom of the tube. Normal results : Male: 40.7 - 50.3% Female: 36.1 - 44.3% Hematocrit (Hct)
  29. 29. High Hematocrit may be due to: •Congenital heart disease •Cor pulmonale •Dehydration •Erythrocytosis •Low blood oxygen levels (hypoxia) •Pulmonary fibrosis •Polycythemia vera Low Hematocrit may be due to: •Anaemia
  30. 30. Erthrocytes Indices •To evaluate the nature of Anaemia, assistance is obtained by calculating standard indices relating to the size of RBCs. •By measuring these indices we can classify anaemia as Microcytic, Macrocytic And Normocytic and Hypochromic and Normochromic. Types MCH MCHC MCV
  31. 31. The Haemoglobin content of erythrocyte is referred to as the Mean Corpuscular Haemoglobin(MCH) expressed in picogram of haemoglobin per cell. MCH = Haemoglobin concentration (g/dl) × 100 RBC in million/mm3 Mean Corpuscular Haemoglobin (MCH)
  32. 32. The concentration of Haemoglobin in the erythrocyte is referred to as the Mean Corpuscular Haemoglobin Concentration.(MCHC) expressed in picogram of haemoglobin per cell. MCHC = Haemoglobin concentration (g/dl) × 100 Hematocrit Mean Corpuscular Haemoglobin Concentration (MCHC)
  33. 33. The average red cell volume is referred to as the Mean Corpuscular Volume(MCV) . It is expressed in cubic microns per cell. MCHC = Hematocrit × 100 RBC in million /mm3 Mean Corpuscular Volume (MCV)
  34. 34. Different types of Anaemia and Indices Types of Anemia MCV MCH MCHC Microcytic Hypochromic Decreased Decreased Decreased Macrocytic Normochromic Increased Increased Normal Normocytic Normochromic Normal Normal Normal
  35. 35. The common causes of Microcytic & Hypochromic Anemia (decreased MCV and MCH) are: •Iron deficiency anemia •Anemia of chronic disease •Thalassemia •Sideroblastic anemia The common causes of Macrocytic Anemia (increased MCV and MCH) are as follows: •Folate or Vit B12 deficiency anemia •Liver disease •Hemolytic or Aplastic anemias •Hypothyroidism •Excessive alcohol intake •Myelodysplastic syndrome
  36. 36. The common causes of Normocytic And Normochromic Anemia (normal MCV, MCH and MCHC) are: •Anemia of chronic disease •Acute blood loss •Hemolytic anemia, such as autoimmune hemolytic anemia, hereditary spherocytosis, or nonspherocytic congenital hemolytic anemia (G6PD deficiency, other) •Anemia of renal diseases.
  37. 37. PLATELET/THROMBOCYTE COUNT The number of platelets in a specified volume of blood. Platelets play a vital role in Haemostasis. Normal range (Adult) =150,000 to 400,000/ cmm of blood. (150 to 400 x 109/ L) Normal range(Children) =150,000-450,000 /cmm of blood. (150-450 x 109/L)
  38. 38. Interpretation of Platelet count THROMBOCYTOSIS: Post operative phase Pregnancy Post partum phase Haemolytic Anemia Trauma Polycythemia vera Chronic myelocytic leukemia THROMBOCYTOPENIA: Acute leukemia Idiopathic thrombocytopenic purpura Aplastic anemia Effect of chemotherapy Hypersplenism
  39. 39. It Measures the time required for hemostatic plug to form. Lack of any clotting factor or platelet abnormalities will prolong the bleeding time. It is used to screen disorders of platelet function and thrombocytopenia Normal Bleeding Time: 2 - 6 minutes Methods are: Duke method and Ivy’s method Bleeding Time
  40. 40. An abnormal Bleeding time- It is usually the result of abnormalities in the structure / abilities of capillaries to contract or abnormalities in the number (Thrombocytopenia) and functional integrity of platelets. Interpretation of bleeding time
  41. 41. •It is the test of the ability of superficial capillaries of the skin and forearm and hands to withstand an increased intraluminal pressure and a certain degree of hypoxia. •It is a clinical diagnostic method to determine hemorrhagic tendency. It is done by occluding the upper veins of the upper arm with a blood pressure cuff for five minutes. Also known as Tourniquet Test/ Rumpel Leede Test Positive result: unequivocal petechiae seen distal to cuff. Negative result: If only 1 or 2 petechiae seen distal to cuff. Capillary Fragility Test
  42. 42. Time required for coagulation to occur in a sample of whole blood outside the body is known as Clotting Time. Normal time- 3 to 7 minutes Method are: • Capillary tube method • Le and white’s test tube method Clotting Time
  43. 43. An abnormal Clotting time- It is usually prolonged in diseases affecting stages of coagulation. It is also increased in:Cirrhosis Hemophilia A and B Factor XI deficiency, Hypofibringenemia and Heparin & Dicumarol therapy. Interpretation of Clotting time
  44. 44. •It is the measure of the rate at which RBCs sediments in a period of one hour. •Also called as Sedimentation Rate or Westergren ESR •It is a common haematology test. •It is a non-specific measure of inflammation. •Also helpful in following progress of some chronic infections (TB and Osteomylelitis) •Done in Westergren pipette Normal ESR Male: 2-5 mm per hr Female: 10- 15 mm per hr Erythrocyte Sedimentation Rate (ESR)
  45. 45. Interpretation of ESR ESR increased: Tuberculosis Osteomyelitis Rheumatic fever Myocardial infarction Rheumatoid arthritis Chronic lung abscess Hodgkin's disease Leukaemia ESR decreased: Congestive cardiac failure Polycythemia Severe dehydration like cholera Physiologic condition where ESR is increased: Pregnancy: After intake of full meal
  46. 46. HEMATOLOGICAL INVESTIGATIONS (not so frequent in dentistry) •Prothrombin Time •Partial Thromboplastin Time •INR
  47. 47. It is the time in seconds that is required for fibrin threads to form in citrated or oxalated plasma. It is used to check the extrinsic pathway factor (F 7) and the common pathway ( F 5, 10 , prothrombin and fibrinogen). Normal range: 11 to 15 seconds Prolonged time indicates abnormal or prolonged Prothrombin time. It gets prolonged when plasma level of any factor is below 10% of its normal value PROTHROMBIN TIME
  48. 48. It is the time in seconds that is required for a clot to form in a sample of oxalated plasma. It is used to check the intrinsic system (8, 9, 11, 12) and the common pathways (5, 10, prothrombin and fibrinogen). Normal range: 25-35 seconds If PTT is prolonged it indicates deficiency of factor 8 or 10 PARTIAL THROMBOPLASTIN TIME
  49. 49. INR: INTERNATIONAL NORMALIZED RATIO The International Normalised Ratio (INR) is a laboratory measurement of how long it takes blood to form a clot. It is used to determine the effects of oral anticoagulants on the clotting system. It is the ratio of Patient’s Prothrombin Time to that of normal Prothrombin time. INR= Patient`s PT Normal PT
  50. 50.  It should be noted that INR is used to monitor Anti coagulant therapy & NOT be used as coagulation screening test  INR values of 5.0 or greater indicate a serious risk of spontaneous bleeding episodes. NORMAL RANGE: 0.8-1.2 (No anticoagulant therapy) 02-03 (On anticoagulant therapy) • Infiltration anesthesia , scaling and root planning INR <3 • Block anesthesia , minor surgery , extraction INR <2 • Major surgeryINR <1.5
  51. 51. OTHER BLOOD TESTS
  52. 52. RENAL TEST Creatinine is a chemical molecule that is present in the serum of the blood. It's produced from another molecule, Creatine, which is a component of muscle. The amount of Creatinine the body produces each day depends on the person's muscle mass. The normal serum Creatinine range for Men= 0.5-1.5 mg/dL. Women is 0.6-1.2 mg/dL
  53. 53. SIGNIFICANCE: When the kidneys are functioning normally, the amount of Creatinine in the serum should remain even. When they're not working properly, the serum Creatinine level increases.
  54. 54. •Blood Urea Nitrogen (BUN) is another measure of wastes (urea) in the blood. •Urea is produced from the breakdown of protein already in the body and protein in your diet. The normal BUN level = 7-20 mg/dL in adults and = 5-18 mg/dL in children. Blood Urea Nitrogen (BUN) SIGNIFICANCE: •A high BUN usually means that kidney function is less than normal, but other factors may affect the BUN level. •Sometimes a low BUN may also mean that not enough intake of protein.
  55. 55. BLOOD GLUCOSE Normal Blood Sugars Level: •A normal fasting (no food for eight hours) 70 and 99 mg/dL •Post Prandial (two hours after eating) upto140 mg/dL •Random Blood sugar level: 70-140mg/dl Diabetes is diagnosed by any one of the following: •Two consecutive fasting blood glucose tests that are equal to or greater than 126 mg/dL •Any random blood glucose that is greater than 200 mg/dL •A 2-hr Oral glucose tolerance test value over 200 mg/dL
  56. 56. Complications of High Blood glucose level include: •Poor wound healing •Infection •Electrolyte imbalance •Diabetic ketoacidosis
  57. 57. Complications of Low Blood glucose level include: •Loss of consciousness(syncope) •Seizure
  58. 58. The most common HIV test, the Enzyme-Linked Immuno Sorbent Assay, or ELISA (also called EIA), is used to detect HIV antibodies in a sample of the blood. HIV TEST
  59. 59. Although HIV tests are very sensitive, they can produce false-positive results. So ELISA HIV tests must be confirmed with another HIV test, such as a Western blot or Indirect immunofluorescence assay (IFA).
  60. 60. Antibodies won't show up in the blood or body fluid immediately after infection. There is a "window period" of six to 12 weeks, and sometimes several months, before the body starts producing antibodies to the virus. So even if tested negative within a few weeks of being exposed to HIV, one should get tested again at three months and six months.
  61. 61. TEST FOR HEPATITIS B It is important to identify the type of hepatitis virus causing infection to prevent its spread and choose the proper treatment since it is transmitted through infected body fluids. It also can be transmitted from a pregnant woman to her child at or near the time of birth. There are several different HBV tests • Hepatitis B surface Antigen (HBsAg) - this tests is done directly for the presence of virus. ` •Hepatitis B core Antibody (HBcAb or anti-HBc) •Hepatitis B surface Antibody (HBsAb or anti-HBs)
  62. 62. Dental Management of Bleeding Disorder
  63. 63. Haemostatic agents LOCAL Mechanical Thermal Chemical SYSTEMIC
  64. 64. LOCAL HAEMOSTATIC MEASURES MECHANICAL METHODS: •Pressure •Use of Haemostats •Suture and Ligations •Embolization of vessels using steel coils, polyvinyl alcohol foam, gel foam, silicon spheres, and methyl methacrylate.
  65. 65. THERMAL METHODS: •Cautery •Electrocautery •Cryosurgery •Argon beam coagulators •Lasers CHEMICAL METHODS: •Astringent agents: Monsel solution and Tannic acid •Bone wax •Thrombin •Gelfoam •Oxycel •Surgicel •Fibrin glue •Adrenaline
  66. 66. SYSTEMIC HAEMOSTATIC MEASURES •Whole Blood •Platelet rich plasma: one unit can raise the platelet count by 7000-10,000 cells/cmm of blood •Fresh frozen plasma: It contain all the coagulation factors. •Cryoprecipitate: Contain factor VIII, XIII and vWB •Adrenochrome monosemicarbazon and ethamsylate
  67. 67. 90% of inherited haemostatic disorder consist of Haemophilia A,B and Von Wilibrand’s disease. MANAGEMENT OF HAEMOPHILIA A and B PATIENTS: Replacement therapy : 1. Platelet concentrate 2. Fresh frozen plasma 3. Factor VIII,IX concentrate : Hemophilia A 4. Factor IX concentrate : Hemophilia B 5. Desmopressin  Antifibrinolytic therapy: 1. Epsilon-aminocaproic acid (EACA, Plaslloid) 2. Tranexamic acid (AMCA, Transamin)
  68. 68. MANAGEMENT OF PATIENTS WITH VON WILLEBRAND DISEASE: Desmopressin Replacement therapy 1. Platelet concentrate 2. Fresh frozen plasma  Antifibrinolytic therapy: 1. Epsilon-aminocaproic acid (EACA, Plaslloid) 2. Tranexamic acid (AMCA, Transamin)
  69. 69. CONCLUSION Reviewing clinical laboratory test results about a patient's condition can provide valuable information for Diagnosis and management of orofacial conditions Guidance on assessing the patient's ability to tolerate the proposed dental treatment A prognosis based on a particular treatment
  70. 70. REFRENCES: •Ganong WF. Review of medical physiology. 21st Edition. Lange medical publishers. 2004. • Cyril KA, Eric N, Norman J. Samson wright’s applied physiology. 13th Edition. Oxford university press. 2002. • Chaudhary SK. Conscise medical physiology. 2nd Edition. New central book agency private limited. 2003. • Taylor JB. Physiological basis of medical practice. 12th Edition. Wavery pvt ltd. 2001. • Kumar CR. Basic pathology. 7th Edition. Elsevier publications. 2003 • Mohan H. Essential Pathology for Dental students. 2nd Edition. Jaypee publications. 2005 • Tandon S. Textbook of Pedodontics. 1st Edition. Paras medical publications. 2003. •Textbook of Oral Medicine. 2nd edition. Paras Publications.2010

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