Luna Hilic Broch
Luna Hilic Broch
Luna Hilic Broch
Luna HILIC
Luna HILIC columns retain a water-enriched layer on the surface of the silica. This water layer facilitates the transfer of polar compounds into the stationary phase for increased retention. Separation is achieved through the partitioning of polar solutes from the high concentration, water-miscible, organic mobile phase into the hydrophilic surface environment. Polar solutes exhibit increased retention, and elute in the order of increasing hydrophilicity.
NEW
Luna HILIC lives up to the exacting standards of quality and customer satisfaction that has been exemplified in the 10 years of the Luna line.
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Table Of Contents
Benefits of HILIC Chromatography
Luna HILIC delivers
Superior retention of polar compounds Increased mass spec sensitivity Increased laboratory throughput and productivity Polar Compound Retention~ ~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~ Page 2-3 Improved Mass Spec Sensitivity~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~ Page 4-5 Increased Sample Throughput~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~~ Page 6-7
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W
Polar Compounds on Luna HILIC
A note on analyte retention and solubility characteristics in HPLC: An analyte must, to some degree, be soluble in or have an affinity for, both the column stationary phase and the mobile phase. This principle is illustrated in the General Chromatographic Performance equation as retention factor or (k), a measure of the degree to which the compound is retained by the column. This critical parameter may be optimized to influence the overall chromatographic separation.
ith HILIC mode techniques, polar compounds receive the highest degree of retention! As such, Luna HILIC will retain the polar compounds that elute near the void in reversed phase chromatography. To effectively illustrate the competencies of HILIC mode chromatography, we have selected nine water-soluble vitamins, demonstrating diverse chemistry and selectivity, for use as probes.
to
9 8
min
12
Luna 5 m HILIC 150 x 4.6 mm 00F-4450-E0 A: Acetonitrile B: Water C: 100 mM Ammonium Acetate, pH 5.8 A/B/C (90:5:5) for 2.5 min to A/B/C (50:45:5) in 7.5 min, hold for 2.5 min. Re-equilibrate @ A/B/C (90:5:5) for 7.5 min. 2.0 mL/min UV @ 260 nm Ambient + 1. p-Aminobenzoic Acid pKa 4.7, H pKa 2.7 logP 0.83 + 2. Nicotinamide H pKa 3.35 logP 0.37 3. Riboflavin pKa 10.2 logP 1.46 4. Nicotinic Acid pKa 4.7, H+pKa 3.0 logP 0.36 + 5. Pyridoxine H pKa 5.6, pKa 8.6 logP 0.77 + 6. Thiamine H pKa 5.5 logP 4.6 7. Ascorbic Acid pKa 4.1, 11.2 logP 1.85 8. Cyanocobalamin pKa 1.59 logP 0.90 9. Folic Acid pKa 2.7, 4.1, 8.9 logP 0.02
Why Vitamins?
Vitamins provide an ideal platform to demonstrate the benefits of HILIC chromatography. The chosen vitamins used in our testing incorporate the following: Broad range of pKa values Variety of functional groups Wide logP range (5.4 units)
The effect of increased polar compound retention can be easily seen through this group of vitamins.
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Because HILIC uses a solvent system that is the reverse of what is common in reversed phase, the peak elution order is reversed on Luna HILIC. Polar/ Hydrophilic compounds that are particularly difficult to retain even on polarembedded reversed phase columns will enjoy maximum retention on HILIC.
App ID 16442
1.2e4 1.1e4
Ribavirin on C18
0.5 ng on column Elutes at void Peak area = 17,996
Column: Dimension: Part No.: Mobile Phase: Flow Rate: Detection: Temperature: Sample: App ID 16343 Gemini 5 m C18 100 x 2.0 mm 00D-4435-B0 Acetonitrile with 0.1 % v/v Formic Acid/Water with 0.1 v/v % Formic Acid (3:97) 0.4 mL/min Mass Spectrometer (MS) (ambient) Ambient 1. Ribavirin (MRM: 245.2/113.2)
App ID 16440
0.2
0.4
0.6
0.8
1.0
1.2
1.4
1.6
1.8
2.0
2.2
2.4
2.6
2.8
min
k = 0.85
0 0.2 0.4 0.6 0.8 1.0 1.2 1.4 1.6 1.8 2.0 2.2 2.4 2.6 2.8
3.0 min
1.8e4 1.7e4
Ribavirin
1.6e4 1.5e4
O NH2 N HO O N N
1.4e4
Highly polar compounds such as Ribavirin may be poorly retained on reversed phase columns HILIC techniques will increase polar compound retention and sensitivity
1.3e4 1.2e4 1.1e4 1.0e4 9000.0 8000.0 7000.0 6000.0 5000.0 4000.0
HO OH
App ID 16441
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T
Increased Sensitivity in LC-MS/MS with Luna HILIC
The analysis of bioanalytical samples in support of clinical and preclinical pharmacokinetic studies requires a highly sensitive analytical methodology, capable of achieving low detection and quantitation limits. Obtaining very low LOD and LOQ levels can be achieved by an increase in the analyte signal, a decrease in the noise, or both. Poor sensitivity is a problem observed for a number of analytes. The two most critical factors of sensitivity in LC-MS/MS are: 1. The chemical and physical properties of the sample
App ID 16335
he increased retention in HILIC allows elution of the analytes outside the suppression region and thus increased detector sensitivity. In addition to the increased retention and sensitivity, HILIC also resolved the compounds with the reverse order of that seen in RPLC. Elution reversal in HILIC can be a benefit when interferences are observed in RPLC.
0.5 ng on column
Increase in sensitivity Nicotine Peak Area 82,900 Nornicotine Peak Area 69,200
Flow Rate: Detection: Temperature: Sample:
1.6e4 1.2e4 1.4e4 1.0e4 8000.0 1.2e4 6000.0 1.0e4 4000.0 8000.0 2000.0 6000.0 0.0 4000.0 2000.0 0.0
1.4e4
Luna 5 m HILIC 100 x 2.0 mm 00D-4450-B0 Acetonitrile /100 mM Ammonium Formate, pH 3.2 (90:10) 0.4 mL/min Mass Spectrometer (MS) Ambient 1. Cotinine (MRM: 177/80) 2. Nicotine (MRM: 163/80) 3. Nornicotine (MRM: 149/80)
0.2
0.4
0.6
0.8
1.0
1.2
1.4
1.6
1.8
2.0
2.2
2.4
2.6
2.8
3.0
3.2
3.4 min
We have illustrated an undesirable combination of these two factors coming together in the reversed phase application to the right. 1. Difficult to retain polar compounds 2. The biological matrix creates an ion suppression zone, or the area in which many of the endogenous compounds in the biological matrix elute - the result is a shortcoming of LCMS/MS commonly referred to as the Matrix Effect.
0.2
0.4
0.6
0.8
1.0
1.2
1.4
1.6
1.8
2.0
2.2
2.4
2.6
2.8
3.0
3.2
3.4 min
Using the Luna HILIC column, we observe an increase in analyte retention away from the suppression zone - effectively decreasing noise. The high organic mobile phase offers more favorable desolvation and ionization conditions, resulting in an increase in analyte signal. By creating these more favorable conditions for both retention and ionization, Luna HILIC columns allow for improved sensitivity in the analysis of bioanalytical samples.
App ID 16345
Gradient:
1.8e4
0.2
0.4
0.6
0.8
1.0
1.2
1.4
1.6
1.8
2.0
2.2
2.4
2.6
2.8
3.0
3.2
3.4 min
8000.0 6000.0
Gemini 5 m C18 100 x 2.0 mm 00D-4435-B0 A: Water with 0.1 % v/v Formic Acid B: Acetonitrile with 0.1 % v/v Formic Acid A/B (97:3) hold 1 min, to (70:30) in 2 min, to (97:3) in 0.01 min, hold for 2.5 min 0.4 mL/min Mass Spectrometer (MS) Ambient 1. Nornicotine (MRM: 149.1/80.1) 2. Nicotine (MRM: 163.3/105.9) 3. Cotinine (MRM: 177.3/80.1)
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0.2
0.4
0.6
0.8
1.0
1.2
1.4
1.6
1.8
2.0
2.2
2.4
2.6
2.8
3.0
3.2
3.4 min
2L
una HILIC allows low level polar metabolites to be retained on column past the critical ion suppression zone, allowing: Increased MS sensitivity Higher signal-to-noise ratio (S/N)
S/N = 20.6
Great MS sensitivity
Column: Dimension: Part No.: Mobile Phase: Flow Rate: Detection: Temperature: Sample:
Luna 3 m HILIC 100 x 2.0 mm 00D-4449-B0 Acetonitrile / 100 mM Ammonium Formate, pH 3.2 (90:10) 0.4 mL/min Mass Spectrometer (MS) Ambient Bamethan
App ID 16443
to
min
S/N = 6.2
Poor MS sensitivity
Column: Dimension: Part No.: Mobile Phase: Flow Rate: Detection: Temperature: Sample: Gemini 3 m C18 100 x 2.0 mm 00D-4435-B0 0.1 % Formic Acid / Acetonitrile (97:3) 0.4 mL/min Mass Spectrometer (MS) Ambient Bamethan
to
min
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ILIC mode allows you to directly inject after sample preparation in high organic eluents and therefore skip the time-consuming evaporation and reconstitution step.
HILIC Workflow
Step 1.
Step 3.
Analysis
S Skip
tep 2
RP Workflow
Sample Preparation LLE SPE PPT
Step 1.
Step 2.
Step 3.
Analysis
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n HILIC chromatography, a 5:1 acetonitrile : water injection solvent constitutes a weak injection solvent. Morphine and metabolites were injected on the Luna HILIC column in a typical sample preparation eluent 5:1 acetonitrile : water and the compounds are well retained and well resolved.
2
App ID 16445
Luna 3 m HILIC 100 x 2.0 mm 00D-4449-B0 A: Acetonitrile / 100 mM Ammonium Formate, pH 3.2 (90:10) B: Acetonitrile / 20 mM Ammonium Formate, pH 3.2 (50:50) A/B (100:0) hold for 1 min to (0:100) in 2 min, A/B (0:100) hold for 1.5 min 0.4 mL/min 5 L Mass Spectrometer (MS) Ambient 1. Morphine 2. Normorphine 3. Morphine-3--Glucuronide
min
n reversed phase chromatography, injecting solutes in typical sample preparation eluents such as 75 85 % organic will result in unfavorable results, such as broad peaks or loss retention. Morphine and metabolites lose all retention and elute in the void.
Co-elution
App ID 16446
2
1 2 3
1
4 min
min min
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Stability
High pH Stability Test
pH = 8.5
Nicotinamide Thiamine
Column: Dimension: Part No.: Mobile Phase: Gradient: Flow Rate: Detection: Temperature: Luna 5 m HILIC 150 x 4.6 mm 00F-4450-E0 A: Water, B: Acetonitrile, C: 100 mM Ammonium Acetate pH 8.5 0:90:10 (A/B/C) to 40:50:10 (A/B/C) in 15 min 1.0 mL/min UV @ 260 nm Ambient
2
Nicotinamide
6
Thiamine
10 min
10 min
Column: Dimension: Part No.: Mobile Phase: Gradient: Flow Rate: Detection: Temperature:
pH = 2.2
Luna 5 m HILIC 150 x 4.6 mm 00F-4450-E0 A: Water, B: Acetonitrile, C: 0.1 %TFA in Water, pH 2.2 0:90:10 (A/B/C) to 40:50:10 1.0 mL/min UV @ 260 nm Ambient
ACN ACN H 2O
OH
ACN
OH O O OH O H2O
H2O
OH
H O
H 2O O H 2O H2O H 2O H2O
HO
10 min
After 7200 column volumes Cyanocobalamin
12
14
OH ACN
10 min
12
14
Addition of TFA
Please note the retention effects caused by the TFA modifier. This weak ion pair reagent associates with the charged groups on the polar vitamins and causes them to become increasingly hydrophobic, REDUCING retention in HILIC mode! In this example, TFA was used to illustrate low pH stability. For recommended buffers, please see the HILIC LC/MS Method Development Strategy on pp. 12-15.
2
0 1 0 1
Batch-to-Batch Reproducibility
3 m
1 2 3 to 4
2 1 2 3 4 5 6
5 m
1 2 3 5 6 4
Batch 1
5 6
Batch 1
to
7 min
Batch 2
Batch 2
3 5 4 6
3 to 4
2 3 4 5 6
5 6
to
7 min
2 3
Batch 3
5 6
2 3
Batch 3
to
to
5 4
App ID 16438
4
1 2 3 4 5 6
07 min
App ID 16340
Columns: Luna 3 m HILIC min Luna 5 m HILIC Dimension: 150 x 4.6 mm Mobile Phase: A: Acetonitrile B: 100 mM Ammonium Formate, pH 3.2 C: Water Gradient: A/B/C (90:10:0) to (50:10:40) in min 15 min Flow Rate: 1.0 mL/min Detection: UV @ 260 nm Temperature: Ambient Sample: 1. PABA 2. Nicotinamide 3. Riboflavin 4. Nicotinic Acid 5. Pyridoxine min 6. Thiamine
Low MS-Bleed
he increased stability of the cross-linked DIOL provides the ultra-low bleed profile required for high sensitivity LC-MS/MS applications.
5.0e7 4.8e7 4.6e7 4.4e7 4.2e7 4.0e7 3.8e7 3.6e7 3.4e7 3.2e7 3.0e7 2.8e7 2.6e7 2.4e7 2.2e7 2.0e7 1.8e7 1.6e7 1.4e7 1.2e7 1.0e7 8.0e6 6.0e6 4.0e6 2.0e6 0.0
0.65 2.30 0.10 1.20 1.45 1.65 1.80 2.05 2.50 3.36
3.91
4.06
4.56 5.36
0.5
1.0
1.5
2.0
2.5
3.0
3.5
4.0
4.5
5.0
5.5 min
A: Water B: Acetonitrile A/B (10:90) for 1.5 min to A/B (50:50) in 2 min, hold 1.5 min, step to A/B (10:90), hold for 5 min
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10
4
App ID 16337
Selectivity
1 2 5 to 4 6 3 0 1 2 2 5 4 6 8 min
SeQuant 5 m ZIC-HILIC Luna 5 m HILIC
10
Conditions same for all columns
Columns: As noted Dimension: 150 x 4.6 mm Mobile Phase: Acetonitrile/100 mM Ammonium Formate, pH 3.2 (90:10) Flow Rate: 1.0 mL/min Detection: UV @ 260 nm Temperature: Ambient Sample: 1. PABA 2. Nicotinamide 3. Riboflavin 4. Nicotinic Acid 5. Pyridoxine 6. Thiamine
to
4
App ID 16431
3 0 2 1 4 6
10
to 5 3 0 2 4 6 6 (Thiamine-no elution) 4
App ID 16432
min
10
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2. Nicotinamide
O
3. Riboavin
HO HO
N
4. Nicotinic Acid
O OH
3.77
OH OH N O NH O
N
3.01
OH
4.77
H2N
3.63 Pro-Vitamin B3 (logP=-0.61, pKa=3.63b)
H3C H3C
Objective
1.
Niacin, B3 (logP=0.25, pKa=3.77a, 3.01b)
N N
Quickly determine applicability of HILIC for your compounds Approximate best separation conditions using set of conditions that provide the most information in the least time Provide the basis for further method optimization, if needed
H2 N
2.69b Vitamin B Complex (logP=0.78, pKa=4.77a, 2.69b)
7.97
2. 3.
5. Pyridoxine
OH
8.60
6. Thiamine
NH2 N N+ N S OH CH3
7. Ascorbic Acid
13.80
Part 1:
O
HO
Method Development
O
OH H3C N
H3C
15.08
HO
14.34
Using set of generic conditions, quickly determine HILIC applicability. Screen for best starting conditions.
5.54
5.58
3.52
HO
HO
8.32
Part 2:
Evaluate Method
N NH N N
2.90
8. Cyanocobalamin
O NH2
9. Folic Acid
NH2
OH
4.12
HO N NH
2.08
Vitamins Profile
The vitamins chosen have a wide scope of functionalities and demonstrate key points of HILIC chromatography well. The chosen vitamins used in our testing incorporate the following: Broad range of pKa values Variety of functional groups Wide logP range (5.4 units)
O CH3 H3C N N
O NH2
O OH
O NH O
Part 3:
Method Optimization
Further optimization towards achieving desired criteria
N Co N
2.68
CH3 CH3 N NH HO O N O OH
O H3 C O P O
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2B 100 mM Ammonium Acetate, pH 5.8: Weigh approx 7.71 g of Ammonium Acetate and dissolve in 1 liter (MQ) water. Add 0.5 mL of acetic acid and mix well. Take 10 mL of the aliquot and measure the pH of the aliquot. Luna HILIC pH 3.2
100
1A
90 80
The buffer solutions recommended in 2A and 2B have been selected based upon:
2A
1B
70
The pH desired to attain separations with polar analytes based upon hydrogen bonding High solubility in eluents with high Acetonitrile content Compatibility with MS detection Luna HILIC pH 5.8
60
1C
2B
50
40
10
12 min
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1
3A
App ID 16430
pH 5.8
Luna HILIC (Cross-linked Diol) 3A
pH 3.2
Luna HILIC (Cross-linked Diol)
3B
App ID 16433
Zwitterion
App ID 16435
3B
Zwitterion
3C
App ID 16434
Silica
App ID 16436
3C
App ID 16437
Silica
Columns: As noted Dimension: 150 x 4.6 mm Mobile Phase: A: Acetonitrile B: Water C: 100 mM Ammonium Acetate, pH 5.8 Gradient: A/B/C (90:5:5) for 2.5 min to A/B/C (50:45:5) in 7.5 min, hold for 2.5 min. Re-equilibrate @ A/B/C (90:5:5) for 7.5 min. Flow Rate: 2 mL/min Detection: UV @ 260 nm Temperature: Ambient Sample: 1. PABA, 2. Nicotinamide, 3. Riboflavin, 4. Nicotinic Acid, 5. Pyridoxine, 6. Thiamine, 7. Ascorbic Acid, 8. Cyanocobalamin, 9. Folic Acid
Columns: (3A) Luna 5 m HILIC (3B) SeQuant 5 m ZIC - HILIC (3C) Luna 5 m Silica (2)
Columns: As noted Dimension: 150 x 4.6 mm Mobile Phase: A: Acetonitrile B: Water C: 100 mM Ammonium Formate, pH 3.2 Gradient: A/B/C (90:5:5) for 2.5 min to A/B/C (50:45:5) in 7.5 min, hold for 2.5 min. Re-equilibrate @ A/B/C (90:5:5) for 7.5 min. Flow Rate: 2 mL/min Detection: UV @ 260 nm Temperature: Ambient Sample: 1. PABA, 2. Nicotinamide, 3. Riboflavin, 4. Nicotinic Acid, 5. Pyridoxine, 6. Thiamine, 7. Ascorbic Acid, 8. Cyanocobalamin, 9. Folic Acid
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Ranking
#1
App ID 16430
Zwitterion pH 5.8
#2
App ID 16433
Silica pH 3.2
#3
App ID 16437
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1. Adding organic modifier 2. Adjusting ionic strength 3. Adjusting initial % organic modifier
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over 10 years of proven reproducibility, you can be confident in your choice to develop methods on Luna
3 m Analytical Columns (mm) 150 x 3.0 00F-4449-Y0 00F-4162-Y0 00F-4248-Y0 00F-4251-Y0 00F-4254-Y0 00F-4256-Y0 00F-4377-Y0 100 x 4.6 00D-4449-E0 00D-4162-E0 00D-4248-E0 00D-4251-E0 00D-4254-E0 00D-4256-E0 00D-4377-E0 150 x 4.6 00F-4449-E0 00F-4162-E0 00F-4248-E0 00F-4251-E0 00F-4254-E0 00F-4256-E0 00F-4377-E0 SecurityGuard Cartridges 4 x 2.0 mm for ID: 2.0-3.0 mm -/10pk AJ0-8328 AJ0-4347 AJ0-4289 AJ0-4286 AJ0-4304 AJ0-4350 AJ0-4301 4 x 3.0 mm for ID: 3.2-8.0 mm -/10pk AJ0-8329 AJ0-4348 AJ0-4290 AJ0-4287 AJ0-4305 AJ0-4351 AJ0-4302
Material Characteristics Packing Material Luna HILIC Luna C5 Luna C18(2)-HST Luna C18(2) Luna C8(2) Luna Phenyl-Hexyl Luna Silica (2) Luna CN Luna NH2 Luna SCX Particle Shape/ Size (m) Spherical 3, 5 Spherical 5, 10 Spherical 2.5 Spherical 3, 5,10,15 Spherical 3, 5, 10, 15 Spherical 3, 5, 10, 15 Spherical 3, 5, 10, 15 Spherical 3, 5, 10 Spherical 3, 5, 10 Spherical 5, 10 Pore Size () 200 100 100 100 100 100 100 100 100 100 Surface Area (m2/g) 200 440 400 400 400 400 400 400 400 400 Carbon Load % 5.7 12.5 17.5 17.5 13.5 17.5 7.0 9.5 0.55 % Sulfur Load End Capping No Yes Yes Yes Yes Yes No Yes No No pH Range 1.5-8.0 1.5-10 1.5-10 1.5-10 1.5-10 1.5-10 1.5-7.0 1.5-11 2.0-7.0
5 m Analytical Columns (mm) 150 x 3.0 Phases HILIC Silica(2) C5 C8 C8(2) C18 C18(2) CN Phenyl-Hexyl NH2 SCX 00F-4450-YO 00F-4043-Y0 00F-4040-Y0 00F-4249-Y0 00F-4041-Y0 00F-4252-Y0 00F-4255-Y0 00F-4257-Y0 00F-4378-Y0 100 x 4.6 00D-4450-E0 00D-4274-E0 00D-4043-E0 00D-4040-E0 00D-4249-E0 00D-4041-E0 00D-4252-E0 00D-4255-E0 00D-4257-E0 00D-4378-E0 00D-4398-E0 150 x 4.6 00F-4450-E0 00F-4274-E0 00F-4043-E0 00F-4040-E0 00F-4249-E0 00F-4041-E0 00F-4252-E0 00F-4255-E0 00F-4257-E0 00F-4378-E0 00F-4398-E0 250 x 4.6 00G-4450-E0 00G-4274-E0 00G-4043-E0 00G-4040-E0 00G-4249-E0 00G-4041-E0 00G-4252-E0 00G-4255-E0 00G-4257-E0 00G-4378-E0 00G-4398-E0
SecurityGuard Cartridges
for ID: 2.0-3.0 mm
4 x 2.0 mm -/10pk AJ0-8328 AJ0-4347 AJ0-4292 AJ0-4289 AJ0-4289 AJ0-4286 AJ0-4286 AJ0-4304 AJ0-4350 AJ0-4301 AJO-4307
4 x 3.0 mm -/10pk AJO-8329 AJ0-4348 AJ0-4293 AJ0-4290 AJ0-4290 AJ0-4287 AJ0-4287 AJ0-4305 AJ0-4351 AJ0-4302 AJ0-4308
If Luna does not provide at least an equivalent separation as compared to a competing column of the same particle size, similar phase and dimensions, send in your comparative data within 45 days and keep the Luna column for FREE.
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