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An evaluation of the transfer of saliva-derived DNA.

International Journal of Legal Medicine, 2012

Study Design

Addressed Question

Tertiary transfer of DNA in saliva

Activity Context

None

Category

Transfer Scenario

Specifications

Bodily OriginContactSurfaceTransfer Sequence

Variables of Interest

deposit surfacedeposition scenariosecondary surfacetertiary surfacepresence of moisture

Stringency of Control

Controlled

Number of Individuals

4

Replicates per Individual and Condition

2

Nucleic Acid

DNA

Bodily Origin

salivaskin (thumbs)skin (palm)

Depositor & Contact

Depositor Characteristics

N/A

Criteria for Shedder Status

N/A

Previous Activities

handwashing with soap

Contact Scenario

primary deposit - drying time - (premoistening of primary or secondary substrate) - secondary transfer - (premoistening of secondary or tertiary substrate) - tertiary transfer - sampling

Primary Substrate

Primary Substrate Type

body part: bare thumbs, gloved thumbs, plastic pens

Primary Substrate Material

LatexPlasticSkin

Deposit

licking or holding in mouth for 30s

Delay

5 or 30 min drying time

Secondary Substrate

Secondary Substrate Type

plastic tubes or (moistened) palms of second individual (body part)

Secondary Substrate Material

PlasticSkin

Secondary Substrate Contact

moderate pressure grip 15s

Further Transfer

Plastic tubes or palms (body part) of third participant, moderate pressure grip 15s

Sampling

Background DNA on Sampled Surface

Negative (Assumed)Present

Sampling Time

direct

Persistence

N/A

Sampling Method

double swabbing

Sampling Area

tertiary substrate

Laboratory Analysis

Extraction

QIAamp DNA mini extraction procedure

DNA Quantification

quantifiler Human DNA Quantification kit (AB), 7500 RealTime PCR system

Input for Profiling

a.p.m.i.

Profiling

AmpFlSTR Identifiler Plus, 3130 xl Genetic Analyzer (28 or 34 cycles LCN in duplicates), GeneMapper ID v3.2 software, threshold: 50rfu

Reference Samples

taken from all participants

Profile Interpretation and Mixture Analysis

comparison to reference profiles, relative contribution according to unique allele peak height

RNA Data Interpretation

N/A

Results

DNA Quantity

mostly not quantifiable

Profile Quality

low proportion of alleles observed

Parameter Used for Comparison

DNA quantity (ng), % alleles detected, relative profile contribution by relative unique allelic peak height (rfu)

Summary of Results

DNA mostly not quantifiable indicating a high DNA loss in tertiary transfer; moisture increases transfer rates, the presence of moisture in the initial step is more relevant than in the subsequent transfer steps; in the absence of moisture, secondary contributor is generally major contributor in profiles, in the presence of moisture the saliva depositor mostly is;

Raised Questions

does further enhancement of sensitivity increase the detection of alleles and show the same trends?

Cautionary Remarks

statistical analysis missing; determination of major or minor contributor in several cases based on 1-2 unique allelic peaks