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Prevalence of human cell material: DNA and RNA profiling of public and private objects and after activity scenarios.

FSI Genetics, 2016

Study Design

Addressed Question

Assessment of the prevalence and composition of human DNA samples on private samples

Activity Context

AssaultManual StrangulationScratching

Category

Background DNA

Specifications

BG on ClothingBG on Skin / Other Body LocationsBodily Origin

Variables of Interest

sample surfacelast owner

Stringency of Control

Reality

Number of Individuals

164 (80 samples from skin, 84 from clothing)

Replicates per Individual and Condition

4

Nucleic Acid

DNARNA

Bodily Origin

skin (hands)skin (neck)trace

Depositor & Contact

Depositor Characteristics

N/A

Criteria for Shedder Status

N/A

Previous Activities

normal activities

Contact Scenario

regular use of items - sampling

Primary Substrate

Primary Substrate Type

body part: skin (neck front and back, left and right hands, fingernails), fabric clothing (winter gloves, trouser legs, shirt armpits)

Primary Substrate Material

CottonDenimFabricLeatherPolyesterSkinSkin and NailVariousWool

Deposit

regular use/activity, wearing

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

tapelift, swabbing with mini-tip swabs (wet: water) for fingernails

Sampling Area

neck front and back, whole hand samples, index middle and ringer finger combined for fingernails, gloves: fingers and thumb areas, trouser legs, t-shirt armpits

Laboratory Analysis

Extraction

DNA/RNA coextraction using QIAamp DNA mini kit and mirVana miRNA isolation kit

DNA Quantification

Quantifiler human DNA Quantification Kit (AB) using an ABI 7900HT real-time PCR system

Input for Profiling

500 pg DNA

Profiling

AmpFlSTR NGM PCR Amplification Kit, 3130XL Genetic Analyzer, GeneMapper ID-X version 1.1.1, threshold: 50 rfu RNA: multiplexes as described in Lindenbergh et al (2012), van den Berge et al (2014), van den Berg et al (2016)

Reference Samples

taken from all individuals

Profile Interpretation and Mixture Analysis

minimum number of known contributors determined by maximum allele count, LoCIM-tool to deduce the most prominent component and comparison to reference profiles, determination of percentage total rfus for each known contributor

RNA Data Interpretation

cell type is scored observed when at least half of the theoretically possible peaks in all replicates are detected

Results

DNA Quantity

neck: 0-5 ng, hands: 0-67.5 ng, fingernails: 0.3-58.6 ng, gloves: 0-2.5 ng, trouser ankles: 0.1-29.0 ng, shirt armpits: 0.0-0.6 ng

Profile Quality

1-5 donors, mostly 2 or 3, donor major contributor in the majority, donor full profile in the majority of cases (except for fingernail samples)

Parameter Used for Comparison

DNA yield, number of contributors, completeness donor profile, non-owner total rfu %, cell types

Summary of Results

higher inter- than intra-individual variation for DNA yield; no differences for gender or fabric types; Non-owner alleles observed in the majority of samples but donor alleles generally substantially higher; owner could not be deduced as major contributor in some cases due to high background alleles; skin observed in almost all samples, other cell types (blood, saliva, vaginal mucosa, nasal mucosa) in <20%; nasal mucosa samples are correlated with relatively high DNA yield

Raised Questions

under which circumstances is non-owner observed as major contributor?

Cautionary Remarks

which sampling locations showed which cell types other than skin n.s.; nasal mucosa not detected in all mRNA multiplex versions used;