High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System .

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High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System www.combisep.com

Transcript of High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System .

Page 1: High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System .

High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System

www.combisep.com

Page 2: High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System .

Introduction

• Massive quantities of ssDNA and ssRNA oligonucleotides are produced daily to support the growth of genomic-related applications

• These DNA products need to be characterized to ensure proper sizing and acceptable batch-to-batch purity

• Traditional slab gel-based methods for characterizing DNA products are time-consuming, labor intensive, not readily automated, and provide relatively poor resolution

• While useful for assessing compound identity, Mass Spectrometry cannot quantitatively assess oligonucleotide purity due to size dependent variations in ionization efficiencies

• As a result, a bottleneck exists for characterizing the purity of ssDNA oligonucleotides

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Capillary Gel Electrophoresis (CGE)

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UV

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• Size-based separation of species possessing a constant mass-to-charge ratio (e.g., denatured SDS-protein complexes, ssDNA oligonucleotides, dsDNA)

• Separation medium is a gel-based sieving matrix; smaller sized species migrate faster

• Throughput for single capillary CGE methods range from 15 min – 100 min per sample; not adequate for high throughput quality control

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Principles of MCE-UV Operation

• UV light passing through the detection window of a 96-capillary array is imaged onto a linear photodiode array detector

• Capillary inlets are arranged 8 x 12 for direct injection from 96-well sample plates• Capillary outlets are bundled to a common reservoir enabling pressure or vacuum to be

applied to the array• Samples are separated by the application of a high voltage with optional vacuum flow• 96 individual CE separations are performed in parallel with simultaneous UV detection

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• CGE-UV is the method of choice for assessing oligonucleotide purity, providing higher resolution and superior quantification vs. slab gels.

• Label-free UV detection provides a low cost, toxic free alternative and improved quantification compared to fluorescent label approaches for ssDNA which may possess size and sequence dependent fluorescent labeling efficiencies

• CGE-UV advantages for characterizing oligonucleotide purity include low sample consumption, high resolving power, direct on-line UV detection and automated operation.

• A proprietary gel sieving matrix (Oligel) has been developed for multiplexed

operation. When analyzed at low M concentrations, single nucleotide resolution can be obtained from 10mer to 80mer oligonucleotide lengths, allowing identification of low level n-1, n-2, etc. impurities.

• Multiplexed CGE-UV provides a nearly 50-fold improvement in sample throughput over single capillary CE methods with a minimal loss in separation performance. A throughput of 96 samples/h is achieved for 80mer length oligonucleotides.

ssDNA Oligonucleotide Analysis by Multiplexed CGE-UV

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Oligo PRO™ System (CombiSep, Ames, IA USA)

• Second generation 96-capillary array CE instrument• Fixed wavelength UV or visible detection• Slide-out stage accommodates four 96-well plates (1 waste, 1 buffer, 2 samples)• System can be interfaced to a robotic arm for unattended well plate exchange

Automatic Tray Handler

Sample Tray #1

Sample Tray #2

Waste Tray

Buffer Tray

Front Access Panel

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Capillary Array Cartridge

LampHousing

HV Power Supply

Syringe Pump

Optical Platform Housing

Capillary Array Detection Window

Inside View of the Oligo PRO™ Instrument

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High Pressure Pump Option for Oligonucleotide Analysis on the Oligo PRO™ Instrument

Oligel MatrixCapillary Conditioning

Solution

A/B Switching Valve

• Pressures up to 400 psi can be applied to the capillary array

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96-Capillary Array Viewed from Detector Position

Capillary Outlets(12 Bundles of 8 Capillaries)

Detection Window(Polyimide coating removed)

Capillary Inlets(Arranged in 8 x 12 Format)

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Capillary Array Inlets Viewed from Below

• Direct injection by voltage from 96-well plates• Working injection volume typically 100 l

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Image of 96-Capillary Array on PDA Detector

• Continuous measurement of UV intensity simultaneously in all 96 capillaries• Absolute light intensity does not have to be equal as the relative absorbance is

measured in each capillary

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Oligo PRO™ Specifications for Oligonucleotide Analysis

Detection • Fixed wavelength UV at 254 nm using mercury lamp and narrow band pass filter

Capillary Array Dimensions • 75 m i.d., 200 m o.d.• Effective lengths 40 cm to 55 cm; ~20 cm fixed length from detector to outlet

Sample Preparation• Typical oligonucleotide working concentration of 1-5 M for a standard EK injection

Sample Injection• Electrokinetic; 100 L working injection volume; -2 to -5 kV for 10 - 20 sec

Multiplexed CGE-UV Operational Conditions• Typical total operating current 0.4 – 0.6 mA (<6 A/capillary)• Field strength ~150 V/cm• Forced air capillary cooling at room temperature

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Contains proprietary mix of polymers and 8 M urea to fully denature oligonucleotides

Low UV background at 254 nm

Low current generation (< 5 A per capillary at 150 V/cm)

Self-coating of capillaries to reduce EOF

Low viscosity to facilitate faster pumping speeds

Single base resolution from 14 – 80mers

Relatively fast separation speed (80mers in ~1 h)

Features of Oligel™ Separation Matrix for Multiplexed CE-UV

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Sample: Desalted 14,15 - 19,20 – 29,30 – 39,40 – 59,60 – 79-80mers

Concentration: 1.5 µM (14-30mers); 0.1 µM (39-60mers); 0.2 µM (79,80mers)

CGE-UV: E = -170 V/cm; Sample injection = -5 kV, 10 s; UV = 254 nm

14,15mer

19,20mer

29,30mer

39,40mer

59,60mer

79,80mer

Separation Resolution of Oligel Sieving Matrix

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96-Capillary Separation of 14-80mers Using Oligel™ Matrix

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Analysis of Unmodified (Top) and Amine-modified (Bottom) 70mers

Sample: Desalted Unmodified, Amine-modified 70mers

Concentration: 5 µM Injection: -3 kV, 15 sCE Run: -140 V/cm, 70 min

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A:B=1:9

A:B=1:1

A:B=1:3

Separation of Various Ratios of Unmodified (A) to Amine-modified (B) 70mers

Sample: Desalted Unmodified, Amine-modified 70mers

Concentration: 5 µM Injection: -3 kV, 15 sCE Run: -140 V/cm, 70 min

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Sample: Desalted, Amine-labeled 70mersConcentration: 8 µMSample Injection: -3 kV, 10 secCE Run: -150 V/cm, 70 min

Multiplexed CE-UV Analysis of Amine-modified 70mers

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Characteristics of Gel Matrices Used in CGE

• Chemical Gels– Cross-linked, chemically linked to the capillary wall: not replaceable– Well-defined pore structure but pore size cannot be varied after

polymerization– Heat sensitive– Particulates can damage gel matrix

• Physical Gels– Not cross-linked, not attached to the capillary wall: replaceable– Entangled polymer networks of linear or branched hydrophilic

polymers– Dynamic pore structure– Heat insensitive

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Permanent coating vs. Dynamic coating

Why: for non-cross-linked gel, EOF reduces separation efficiency

How to reduce the EOF?Permanent coating:– Chemical bonding to the capillary wall– Non-replaceable– Limited life time

Dynamic coating:– Physical bonding (hydrophobicity and charge)– Replaceable

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High Pressure Pump Option for Oligonucleotide Analysis on the Oligo PRO™ Instrument

Oligel MatrixCapillary Conditioning

Solution

A/B Switching Valve

• Pressures up to 400 psi can be applied to the capillary array

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Operation Flow Chart

Fill Gel Separation Separation Separation

(400 psi)(3 to 4 hours)

(~1 hour)

Once a week: Conditional Solution + Gel Fill (~4 hours)

Total of ten separations

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Oligonucleotide Analysis : Reagent Cost per Sample

DN-415-0250 Oligel ssDNA Gel, 250 ml  

List Price: € 280 Volume Consumed 20 ml/day + 10 ml/run

  Plates per Day 6

  Samples per Day 576

  Cost per sample (Est.) €0.15

  Plates per Day 10

  Samples per Day 960

  Cost per sample (Est.) €0.14

DN-465-1000 ssDNA Oligel Buffer, 1000 mL  

List Price:€102 Volume per Day (ml) - up to 10 runs 106

  Samples per Day (6 plates) 576

  Cost per sample (Est.) €0.02

  Samples per Day (10 plates) 960

  Cost per sample (Est.) €0.01

DN-475-1000 Capillary Conditioning Solution, 1000 mL  

List Price: €153 Volume (ml) per week (Est.) 250

  Samples per Day (6 plates) 576

  Cost per sample (Est.) €0.01

  Samples per Day (10 plates) 960

  Cost per sample (Est.) €0.01

  Total Reagent Cost per Sample (6 plates/576 samples/day) €0.18

  Total Reagent Cost per Sample (10 plates/960 samples/day) €0.16

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Oligonucleotide Analysis : Capillary Cartridge Cost per Sample

Calculation assumes :1. cost per capillary array = €61942. Operating days per week = 5 days/wk

Samples per day Plates per day

Capillary Lifetime (weeks)

12 16 20 25 36 52

96 1 1,08 € 0,81 € 0,65 € 0,52 € 0,36 € 0,25 €

192 2 0,54 € 0,40 € 0,32 € 0,26 € 0,18 € 0,12 €

288 3 0,36 € 0,27 € 0,22 € 0,17 € 0,12 € 0,08 €

384 4 0,27 € 0,20 € 0,16 € 0,13 € 0,09 € 0,06 €

480 5 0,22 € 0,16 € 0,13 € 0,10 € 0,07 € 0,05 €

576 6 0,18 € 0,13 € 0,11 € 0,09 € 0,06 € 0,04 €

672 7 0,15 € 0,12 € 0,09 € 0,07 € 0,05 € 0,04 €

768 8 0,13 € 0,10 € 0,08 € 0,06 € 0,04 € 0,03 €

864 9 0,12 € 0,09 € 0,07 € 0,06 € 0,04 € 0,03 €

960 10 0,11 € 0,08 € 0,06 € 0,05 € 0,04 € 0,02 €

1248 13 0,08 € 0,06 € 0,05 € 0,04 € 0,03 € 0,02 €

1920 20 0,05 € 0,04 € 0,03 € 0,03 € 0,02 € 0,01 €

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Other Technologies

• Slab Gel• Single column capillary electrophoresis• Mass Spectrometers• HPLC

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Slab Gel

• Multiple samples analysis• Good resolution• Very labor intensive• Difficult to document the image• Semi-quantitation • Long separation time• Acrylamide

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Single Column Capillary Electrophoresis

• Similar resolution as in Oligo PRO™• Better reproducibility• Slow (~96 times slower)• Sample cost: higher due to the use of coated capillary (limited

life time)

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Mass Spectrometers

– MALDI (matrix assisted laser desorption ionization)• Size determination up to 60’mers• Difficult for quantification

– Electrospray ionization • Size determination up to 120’mers• Relatively slow: a couple minutes per sample• Difficult for quantification

– HPLC-MS• Size determination & quantification• Slow: half hour to an hour per sample

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HPLC (Ion Exchanged Chromatography)

• Quantitation measurement• Separation up to 40’mers• Slow: half hour per sample• Separation not completely based on size• Better reproducibility

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Impurity Screening of an Amine-modified 70mer Sample

• Approximate % Purity of main peak is 39.1%

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CombiSep and IDT Poster Co-Winners of Best Poster at Tides 2005 Conference

The poster titled “Comparisons between Multiplexed, Absorbance-Based Capillary Electrophoresis, Capillary Electrophoresis, and Ion Exchange Chromatography for Analysis of n-1 Oligonucleotide Impurities” by Wei Wei, Ho-ming Pang, Dennis Tallman, and Jeremy Kenseth of CombiSep, Inc and Lisa Bogh of Integrated DNA Technology was recently selected as the co-winner of the best poster at Tides 2005. The Tides Conference is an industry event for manufacturing and development of oligonucleotide and peptide products. The meeting was held May 1st – 5th, 2005 at the Boston Convention & Exhibition Center.

The poster award was sponsored by BioProcess International. The selection criteria was based on novelty, applicability, and clarity of data presented.

Co-Winner Best Poster at Tides 2005

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50:50 Mixture of 29mer:30mer by multiplexed CE-UV, CE-UV, and IEC

• IEC method was unable to provide resolution of n-1 species

Multiplexed CGE

Single Capillary CGE

Ion Exchange HPLC

70 min = 96 Samples

25 min = 1 Sample

25 min = 1 Sample

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50:50 Mixture of 39mer:40mer by multiplexed CE-UV, CE-UV, and IEC.

• IEC method was unable to provide resolution of n-1 species

Multiplexed CGE

Single Capillary CGE

Ion Exchange HPLC

70 min = 96 Samples

27 min = 1 Sample

26 min = 1 Sample

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50:50 Mixture of 49mer:50mer by multiplexed CE-UV, CE-UV, and IEC.

• All methods could provide resolution of n-1 species

Multiplexed CGE

Single Capillary CGE

Ion Exchange HPLC

70 min = 96 Samples

30 min = 1 Sample

28 min = 1 Sample

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50:50 Mixture of 59mer:60mer by multiplexed CE-UV, CE-UV, and IEC.

• IEC method was unable to provide resolution of n-1 species• IEC provided no n-1 resolution at 70mer, 80mer lengths• The CGE methods resolved n-1 at 70mer, 80mer lengths

Multiplexed CGE

Single Capillary CGE

Ion Exchange HPLC

70 min = 96 Samples

38 min = 1 Sample

30 min = 1 Sample

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Separation of 36mer and 37mer ssRNA Oligonucleotides

Sample: Two RNA oligonucleotides (36mer, 37mer) were obtained from IDT. The 36mer sequence was 3’-CAGGGACAAGCCCGCCGUGACGAUCUCUAAACAAGC-5’; the 37-mer had an additional A residue on the 3’ end. Samples were diluted to ~ 1 M in water.

Capillary Array: 75 m i.d., 150 m o.d.; 55 cm effective/80 cm total length

CGE: E = 150-170 V/cm. Sample injection: -2 kV, 15 sec

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Oligo PROTM Analyzer System

• Multiplexed CE-UV system designed and optimized specifically for oligonucleotide analysis and QC

• Improved ease-of-use and automation

• Enhanced data analysis and report generation capabilities designed with feedback from scientists directly engaged in oligo production

• Launched in May 2006

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Summary

• Multiplexed CGE-UV provides a powerful method for oligonucleotide purity analysis, providing superior resolution, throughput and automation compared to slab gel methods

• Only minimal sample preparation is required for analysis

• The developed Oligel™ matrix is capable of achieving single base resolution from 14-80mers in about 1 h

• Multiplexed CGE-UV provides much higher sample throughput and superior resolution to HPLC methods. The standard IEC method could not resolve n-1 species at 30mer, 40mer, or above 60 mer lengths

• RNA oligonucleotides as well as dsRNA duplexes can be analyzed for purity in addition to DNA oligonucleotides

Page 39: High Throughput Oligonucleotide Analysis Using the CombiSep Oligo PRO™ System .

Details of Disruptive Technologies

Contacts

William Amoyal (Sales and Marketing Director)

Franck Do Vale (Technical Director)

Disruptive Technologies

3 Allée des Camélias

94440 Villecresnes, France

Mobile: +33 (0)6 98 64 98 81

Email: [email protected]

Web: www.disruptechno.com