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Observations of DNA transfer within an operational Forensic Biology Laboratory.

FSI Genetics, 2016

Study Design

Addressed Question

the amount of background DNA deposited by individuals in a regularly frequented environment

Activity Context

Professional

Category

Background DNA

Specifications

BG in Professional EnvironmentIndividual Characteristics

Variables of Interest

Surfaces sampledPeople regularly frequenting areas

Stringency of Control

Reality

Number of Individuals

>29

Replicates per Individual and Condition

106

Nucleic Acid

DNA

Bodily Origin

trace

Depositor & Contact

Depositor Characteristics

individuals working in a variety of roles with in the biology floor at FSSA

Criteria for Shedder Status

high or low ‘average’ amount of shedding over an extended period of time, by taking a sample that is a snap shot of that individual’s occupancy of the environment over many years

Previous Activities

regular activities

Contact Scenario

regular activities within FSSA lab

Primary Substrate

Primary Substrate Type

various surfaces: fridge handles, lab coat, elevator button, light switch, microscope handle, pipettes, centrifuge, workstation, forceps, scissor, heat blocks, pens, bench tops, draws, trolleys, chairs, calculators, computers, mice, keyboards, phones, printer, kitchen items (tools, personal items)

Primary Substrate Material

MetalPlasticVariousWood

Deposit

regular use/activity

Delay

N/A

Secondary Substrate

Secondary Substrate Type

N/A

Secondary Substrate Material

N/A

Secondary Substrate Contact

N/A

Further Transfer

N/A

Sampling

Background DNA on Sampled Surface

Sampled

Sampling Time

direct/delayed

Persistence

N/A

Sampling Method

popule swabs soaked with isopropanol for non-porous surfaces, tapelifts for porous surfaces

Sampling Area

depending on item, mostly in area most likely touched

Laboratory Analysis

Extraction

DNA IQ system (Promega) in-house validated protocol, Multiprobe II Forensic Workstation

DNA Quantification

Quantifiler Human DNA Quantification Kit (Thermo Fisher), ABI PRISM 7000/7500 SDS

Input for Profiling

a.p.m.i.: 15 µl, max. 1 ng

Profiling

GlobalFiler, ABI PRISM 3130xI Genetic Analyzer, GeneMapper ID-X, Threshold 30 or 100 rfu (for >4 person mixtures)

Reference Samples

taken from 29 individuals working in the building

Profile Interpretation and Mixture Analysis

independent analysis of minimum number of contributors by two individuals, analysis in STRmix calculating an LR for the inclusion of each individual

RNA Data Interpretation

N/A

Results

DNA Quantity

average 0.2 ng/µl in non-sensitive, 0.008 ng/µl in sensitive areas

Profile Quality

n.a., higher contributor number in non-sensitive areas

Parameter Used for Comparison

DNA yield, minimum number of individuals, inclusionary LR

Summary of Results

DNA of individuals is more often found in the individual's immediate environment and is less often associated with items found in areas they do not frequent; there is a trend of finding more DNA in areas that people more often frequent; cleaning regime: non-sensitive areas and highly frequented areas contain more DNA and more complex profiles; comparison between two individuals performing comparable activities in comparable laboratory areas: one individual detected a lot more often and with higher LRs than the other one -> intraindividual shedding differences observed resulting from an averaged shedding behavior over a long deposition time;

Raised Questions

variability of LR? Trend towards neutrality with increasing number of contributors not observed

Cautionary Remarks

DNA yields not comparable due to inconsistent sampling method and area; observations of a consistent shedder status based on two individuals