基于epMotion 5075t及KAPA文库定量试剂盒的全自动NGS文库...1
基于epMotion 5075t及KAPA文库定量试剂盒的全自动NGS文库定量操作
Automated KAPA® Library Quantifcation Kit with the epMotion® 5075t
Maud Brasseur¹, Jennifer Pavlica², Marsha McMakin², Sandrine Hamels¹
¹Eppendorf Application Technologies S.A., Namur, Belgium
²Roche Sequencing & Life Science, Wilmington, USA
Abstract
Next-Generation Sequencing (NGS) is a high-throughput method that
enables highly parallelized sequencing of multiple libraries, prepared
from both DNA and RNA samples. Bolstered by growing applications, such
as the whole genome, whole exome, and gene expression analyses, NGS is
gaining importance and becoming a standard procedure in many
laboratories.
The quantifcation of NGS libraries prior to sequencing is essential to
obtain reliable results and optimal sequencing performance. This
Application Note demonstrates the capability of the epMotion 5075t
liquid handling system to automate with high accuracy and high precision
a complete qPCR assay setup using the KAPA Library Quantifcation Kit
including library dilution steps.
Introduction
Accurate and precise quantifcation of the number of amplifable molecules
in a library is an essential step in sequencing workflows. It ensures
consistent and optimal cluster densities, as well as equivalent
representation of each library when sequencing in multiplex. Inaccurate
quantifcation can result in decreased sequence quality metrics,
inefcient flowcell use, and additional sequencing required for
underrepresented samples – all of which translates to wasted time and
money.
A quantitative PCR (qPCR) approach, such as the KAPA Library
Quantifcation Kit, is the gold standard for NGS library quantifcation
and is the only method that accurately measures the number of amplifable
molecules that have the ability to cluster. Additionally, this method
has the sensitivity and broad dynamic range for accurate quantifcation
of very
dilute and PCR-free libraries.
Performing an accurate qPCR assay manually in a high throughput setting
becomes difcult and time consuming, and the use of an automated liquid
handling platform is strongly recommended to reduce the risk of human
error and increase the reliability of results. The Eppendorf epMotion®
family of automated pipetting systems is an essential tool for many
laboratories looking to achieve consistent results. The epMotion 5075t
and other models in the Eppendorf family pipette volumes ranging from
0.2 µL to 1 mL with efciency and accuracy.
The reliability of qPCR results is highly related to the accuracy and
precision of liquid handling in both reaction setup and library
dilution. Accuracy and precision are two terms that are often used
interchangeably, but are actually differentiated. Accuracy refers to how
close a measurement is to a true value, while precision refers to how
close repeat measurements are to each other and is thus a measure of
reproducibility. This Application Note presents experimental results
aimed at verifying the accuracy and precision of the KAPA Library
Quantifcation Kit processed on the epMotion 5075t compared to manual
handling.
Materials and Methods
Materials
qPCR – Accessories
> LightCycler® 480 Sealing Foil (Roche, cat # 04 729 757 001)
> LightCycler® 480 Instrument, 96-well (Roche, cat # 05 015 278 001)
> Centrifuge MiniSpin®, non-refrigerated, with Rotor F-45-12-11, 230 V/50 – 60 Hz (Eppendorf, cat # 5452000010)
> Centrifuge 5810 R (IVD), refrigerated, without rotor, keypad, 230
V/50 – 60 Hz (Eppendorf, cat # 5811000015) qPCR – Reagents
> KAPA Library Quantifcation Kit for Illumina® platforms (KAPA Biosystems, cat # 07960336001)
> KAPA Library Quantifcation Dilution Control Kit for Illumina® platforms (KAPA Biosystems, cat # 07960417001)
> UltraPure™ 1M Tris-HCl, pH 8.0 (Thermo Fisher®, cat # 15568025)
> Water, Sterile, Nuclease-free, Biotechnology Grade (VWR, cat #
E476)
Methods
KAPA Library Quantifcation Kit contains all reagents required for
quantifcation of NGS libraries for Illumina® sequencing, including KAPA
SYBR® FAST qPCR Master Mix (2X), a Primer PreMix (10X) containing two
primers based on Illumina P5 and P7 oligo sequences (Primer 1: 5’-AAT
GAT ACG GCG ACC ACC GA-3’ and Primer 2: 5’-CAA GCA GAA GAC GGC ATA
CGA-3’) and six ready-to-use DNA standards corresponding to a 10-fold
dilution series. Standards consist of a linear, 452 bp dsDNA fragment
flanked by qPCR primer binding sites. A KAPA Library Quantifcation
Dilution Control, referred to asDNA Standard 0, is a 200 pM solution of
the same linear, 452 bp dsDNA fragment. It is available for purchase
separately and can be used to characterize impact of liquid handling on
assay accuracy.
The epMotion was programmed to perform NGS library sample dilution and
qPCR setup in one method. Reactions were set up according to Table 1 and
thermocycled according to Table 2 using a LightCycler® 480 instrument
(96 well). Template-free negative controls were included.
Manual and automated standard curves were generated using triplicate reactions for each standard. epMotion sample dilution accuracy was assessed using DNA Standard 0 diluted 1:10,000, as well as two NGS libraries diluted 1:10,000; 1:100,000; and 1:1,000,000. The same stock of reagents and samples were used in both manual and automated processes. The qPCR plate layout is illustrated on Figure 1.
Figure 1: qPCR plate layout.
Figure 2: epMotion 5075t worktable for sample dilution and qPCR setup with the KAPA Library Quantifcation Kit for Illumina® platforms.
Before starting the program, the epMotion surfaces and tools were
cleaned using a DNA decontamination solution “DNA Erase” and treated
with UV-light for 15 minutes. The work table of epMotion 5075t
instrument is equipped as in Figure 2.