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Chapter 5: Serology Techniques Section 5.1 only  Forensic Serology = Detection and identification of bodily fluids  Enzymatic assays ▪ Blood: peroxidase in heme group of hemoglobin ▪ Semen: acid phosphatase ▪ Saliva: amylase  Antigen-antibody assays ▪ Primary binding assays ▪ Secondary binding assays Forensic Biology by Richard Li 2  Enzymatic assays  Kastle-Meyer test for blood ▪ Tests for presence of peroxidase activity ▪ Peroxidases break down hydrogen peroxide to water and oxygen free radicals (O-) ▪ Oxygen free radicals are strong oxidants and strip hydrogens off the K-M reagent (oxidize it) ▪ The reduced form of K-M is colorless but the oxidized form is bright pink ▪ Not the same dark red color of blood 3 4  Method ▪ ▪ ▪ ▪ ▪ Moisten Q-tip swab in distilled water Lightly touch suspected blood stain with tip of Q-tip Add one drop K-M reagent Add one drop hydrogen peroxide Look for fast color change to bright pink 5  Limitations  False positive reactions ▪ Any strong oxidizing agent (e.g. bleach) ▪ Will oxidize K-M reagent even in the absence of peroxidase ▪ Any substance with peroxidase activity ▪ Bacteria ▪ Plants  Not species-specific ▪ Reacts with blood from any animal  Sensitivity (too high?) ▪ Will detect blood in urine, saliva, and other body fluids if trace amounts are present 6  Enzymatic assays  AP test for semen ▪ Tests for presence of acid phophatase activity ▪ AP liberates naphthol from alpha-naphthol and the naphthol then reacts with brentamine to form a purplecolored dye α-naphthyl acid phosphate monosodium salt sodium phosphate + naphthol Acid phosphatase napthol + Brentamine Purple azo dye Coupling reaction 7  Method ▪ Spray a Whatman paper circle with distilled water ▪ Lay the paper down over the suspected semen stain ▪ Leave in contact with stain 30-60 seconds ▪ Remove paper circle from stain and spray with AP spot solution ▪ Look for a rapid color change to purple 8  Limitations  False positive reactions ▪ Any substance with acid phophatase activity ▪ Bacteria ▪ Plants ▪ Vaginal fluid  Not species-specific ▪ Reacts with semen from any animal ▪ Not usually a big problem in forensic casework ▪ Animal sperm are morphologically distinct from primate sperm under the microscope 9 10  Enzymatic assays  Amylase test for saliva ▪ Tests for presence of amylase enzyme ▪ Amylase is present in saliva and small intestine ▪ Salivary amylase = ptyalin ▪ Pancreatic amylase = amylopsin  Breaks down starch to simple sugars  Two types of starch: amylose and amylopectin ▪ Amylose changes color from clear to deep blue-black in the presence of iodine 11 amylose amylopectin Forensic Biology by Richard Li 12  Method ▪ Spray a Whatman paper circle with solution of soluble starch ▪ Lay the paper down over the suspected saliva stain ▪ Leave in contact with stain for 20 minutes ▪ Incubate in a 37 deg moisture chamber for 1 hour, then dry ▪ Spray with iodine and look for a lack of color change to deep blueblack 13  Limitations  False positive reactions ▪ Any substance with amylase activity ▪ Bacteria ▪ Plants ▪ Vomit  Not species-specific ▪ Reacts with saliva from any animal that produces it ▪ Not usually a big problem in forensic casework ▪ Cats and dogs do not produce amylase 14  Enzyme-Linked Immunosorbent Assays (ELISA) is most common type used  Very sensitive  Colorimetric or fluorometric signal is proportional to the amount of bound antigen  Often performed in wells  Detected by color change  Two methods: ▪ Well ▪ Cassette 15 16  Immunochromatographic ELISAs  Rapid and simple test  Used as screening test in the field for seminal and     saliva stains and for species identification High-dose effect Highly sensitive (too sensitive?) Specificity still under debate We will perform these in lab 17 human semenogenlin monoclonal goldlabeled murine anti human semenogelin antibody to epitope 1 monoclonal unlabeled murine anti human semenogelin antibody to epitope 2 polyclonal unlabeled goat anti murine antiglobulin T Positive RSID™ semen test C T 18 Negative RSID™ semen test C T 19