Identification of Spermatozoa From Challenged Samples Chelsea Ellis and Reena Roy, Ph.D ABSTRACT...

Identification of Spermatozoa From Challenged SamplesChelsea Ellis and Reena Roy, Ph.D

ABSTRACT This research involved the detection of human spermatozoa from challenged samples using fluorescent staining with Sperm HY-LITERTM. The fluorescently stained human male cells were detected using fluorescence microscopy without the aid of computer software. Extracted spermatozoa were stained with reagents contained in SPERM HY-LITER™ kit developed by Independent Forensics. The spermatozoa deposited on various substrates, subjected to various conditions were identified using a Leica DM2500 P fitted with a Prior Lumen 200 Fluorescence Illumination System.

MATERIALS AND METHODS

RESULTS

CONCLUSION•Negative controls showed no transfer of spermatozoa in this experiment (controls in the same bag)

•Fabrics washed with hot water and detergent yielded less spermatozoa than fabrics washed with cold water

•Spermatozoa binds more tightly to cotton fabric than black leather

•This method can accurately and efficiently detect spermatozoa without a fluorescent microscope or an expensive computer software

•The results obtained from this research indicates that a manual method of detection of fluorescently stained spermatozoa can benefit forensic biology laboratories.

A Leica DM2500 P microscope was used for the detection of the samples on the slides. The fluorescently labeled spermatozoa were identified with a Prior Lumen 200 Fluorescence Illumination System attached to the Leica DM2500 P. The human spermatozoa were searched for manually without the aid of any computer software or microscope stage.

Normal human semen was diluted with water and deposited on fabrics such as leather, denim, fleece, polyester, and polyester-cotton blend. Together, the fabrics deposited with semen and fabrics without semen (negative control) were subjected to two different types of wash cycles (hot or cold) and with and without Tide® detergent. The fabrics were dried at room temperature overnight and then extracted in 20 ul of water for 30 minutes. The extracted semen was deposited on a 25x75 mm, 1.0 mm thick, pre-cleaned VWR Scientific Micro slides and stained with SPERM HY-LITER™ reagents.

Substrate Body Fluid Time Left at RT Wash Time Extraction Time Extracted In Results

Denim 1µL Human Semen Overnight Cold Wash Cycle 30 Minutes 20µL Water Many Observed




White Polyester 1µL Human Semen Overnight Cold Wash Cycle 30 Minutes 20µL Water Many Observed




Black Leather 1µL Human Semen Overnight Cold Wash Cycle 30 Minutes 20µL Water Few Observed



Black Leather 1µL Human Semen Overnight Cold Wash Cycle 30 Minutes 20µL Water Several Observed

Black Fleece 1µL Human Semen Overnight Cold Wash Cycle 30 Minutes 20µL Water Several Observed




Substrate Body Fluid Time Left at RT Wash Time Extraction Time Extracted In Results

Denim 5µL Human Semen Overnight Hot Wash Cycle 30 Minutes 20µL Water A few Observed

Denim 5µL Human Semen Overnight Hot Wash Cycle+ Detergent 30 Minutes 20µL Water A few Observed

Denim 10µL Human Semen 5 days Hot Wash Cycle 30 Minutes 50µL Water Many Observed

Denim 10µL Human Semen 5 days Hot Wash Cycle+ Detergent 30 Minutes 50µL Water A few Observed

Cold Water Without Detergent

Hot Water With and Without Detergent

Sperm HY-LITERTM

Black Leather

Sperm HY-LITERTM

Cotton

Sperm HY-LITERTMBlack Fleece

Sperm HY-LITERTM

White Polyester

Sperm HY-LITERTM

Cotton

KPIC Human Spermatozoa

KPIC Bull Spermatozoa

KPIC Human Spermatozoa

Date post:	17-Jan-2016
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Identification of Spermatozoa From Challenged Samples Chelsea Ellis and Reena Roy, Ph.D ABSTRACT...

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