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mRNA-based skin identification for forensic applications

International Journal of Legal Medicine, 2011

Study Design

Addressed Question

persistence of mRNAs in touch samples

Activity Context

None

Category

PersistenceRecovery

Specifications

Persistence with TimeRNA Profiling

Variables of Interest

storage time

Stringency of Control

Controlled

Number of Individuals

5

Replicates per Individual and Condition

1-2

Nucleic Acid

RNA

Bodily Origin

skin (fingertips)

Depositor & Contact

Depositor Characteristics

good, medium and poor shedders

Criteria for Shedder Status

determined by the overall success rate of amplification of the target and reference genes (data n.s.)

Previous Activities

N/A

Contact Scenario

deposit of thumbprint - delay - sampling

Primary Substrate

Primary Substrate Type

slide

Primary Substrate Material

Glass

Deposit

thumbprint

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

Negative (Confirmed)

Sampling Time

delayed

Persistence

time: 6.5 months under dust-free, non-humid conditions

Sampling Method

Pinpoint Slide RNA Isolation System

Sampling Area

full thumbprint

Laboratory Analysis

Extraction

Pinpoint Slide RNA Isolation SystemII

DNA Quantification

RNA: NanoDrop ND-1000 spectrophotometer

Input for Profiling

5-11 µl total RNA for cDNA synthesis, 5µl of undiluted cDNA for RNA profiling

Profiling

RNA: qPCR of: CDSN, KRT9, LOR and ACTB

Reference Samples

N/A

Profile Interpretation and Mixture Analysis

N/A

RNA Data Interpretation

'dCt for skin-specific mRNA markers <2.7 counts as skin identified

Results

DNA Quantity

N/A

Profile Quality

mostly all markers detected, KRT9 not detected in 40% of samples

Parameter Used for Comparison

Ct, dCt

Summary of Results

no significant difference in expression signals observed for any of the mRNA markers from thumbprints sampled directly or 6.5 months after deposition; KRT9 shows a slight (not statistically significant) trend of decreasing detection levels indicating that KRT9 transcript might be more susceptible to time-wise degradation

Raised Questions

longer time intervals should be investigated

Cautionary Remarks

even though not statistically significant: more samples with higher dCt value after 6.5 months: is ACTB more stable than other markers?