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HPLC
( Basic Principles, Operations and
Maintenance and Troubleshooting )
Alimuzzaman
Sr. Officer, R&DA
Incepta pharmaceuticals Ltd, Dhaka
Bangladesh
Mob : 8801726041712
HPLC in recent time
Characterization
Instrumentation
Basic Configuration of HPLC
Separation Modes
Reversed Phase HPLC System
Reversed Phase HPLC System
Peak Parameters
Factors!!!
Column Dead Volume
Worn
Exercise!!
Answer!!!
Normal Phase HPLC System
Normal Phase HPLC System
Converting Normal Phase to Reverse
Phase and Vice versa
To convert a normal phase system/column to a reversed phase
system/column, flush with a solvent that is miscible with both the current
normal phase solvents and ideally
Normal Phase : Hexane/Ethyl Acetate
Flush : IPA then Methanol
Finally : 50:50 Methanol/Water
Reversed Phase : Buffered Aqueous Methanol
To convert a reversed phase system/column to a normal phase
system/column, follow a similar path to the one listed previously, but in
reverse, for example,
Reversed Phase : Buffered Aqueous Methanol
Flush : 50:50 Methanol/Water
Methanol then IPA
Normal Phase : Hexane/Ethyl Acetate
HILIC System
Various HPLC Detectors
UV-Vis Detector
Solvent cut off-value
PDA Detector
PDA Detector
Evaporating Light Scattering
Detector (ELSD)
ELSD Mechanism
Maintenance
HPLC System Maintenance Strategy
Individual HPLC Module
Preventive Maintenance
Possible problems from the Pumps
Replacement and cleaning of suction
filter
Auto sampler common problems
UV-VIS and PDA detector common
Problem
When to Change the Lamp
Good Laboratory Practice for HLPC
1. Preparation of Solvents :
Correct solvent preparation is very important. It can save vast
amounts of time spent troubleshooting spurious peaks, base-line
noise etc.
2. Quality :
All reagents and solvents should be of the highest quality. HPLC
grade reagents may cost slightly more than lower grade reagents,
but the difference in purity is marked. HPLC grade reagents contain
no impurities to produce spurious peaks in a chromatogram baseline whereas
AR grade reagents do contain trace levels of impurity, which may
produce spurious baseline peaks.
Important: Do not store HPLC grade water in plastic containers. Additives in the plastic may
leach into the water and contaminate it. Always store HPLC grade water in glass containers
3. Buffers :
All buffers should be prepared freshly on the day
required. This practice ensures that the buffer pH is
unaffected by prolonged storage and that there is no
microbial growth present. Changes in pH and microbial
growth will affect chromatography.
If buffer solutions are stored, be aware that they have a
finite lifetime. Refer to pharmacopoeia monographs or
similar for further guidance on buffer shelf life.
Good Laboratory Practice for HLPC
4. Filtration :
Ideally, all HPLC solvents should be filtered through a 0.45
μm filter before use. This removes any particulate matter that
may cause blockages. After filtration, the solvents should be
stored in a covered reservoir to prevent contamination with dust
etc. Filtering HPLC solvents will benefit both your
chromatography and the wear and tear of the HPLC system.
Pump plungers, seals and check valves will perform better and
lifetimes will be maximized.
Good Laboratory Practice for HLPC
Good Laboratory Practice for HLPC
Wash
Pump
Injector
Flow Cell
Column
Hundred Problems
Thousand Solutions
Please DO!!!
References
• Maintaining and trouble shooting HPLC- David J. Lunser, copyright 1981 by Wiley and sons
Inc.
• Modern HPLC for practicing Scientist- Micheal W. Dong.
• E.L Jhonson and R. Stevenson, Basic liquid Chromatography, Varian Associates, Palo Alto,
California -1978.
• L.R Snyder and J. J. Kirkland, Introduction to modern Liquid Chromatography, 2nd edition.
• J. K Walker M.T. Jackson Jr., and J. B. Maynard-Chromatography System- Maintenance and
Trouble Shooting, 2nd edition.
• Trouble Shooting in HPLC –Agilent Technologies.
• Theory and Principle of HPLC –Tranining Module, Shimadzu Asia Pacific Pte Ltd, Singapore
Part – I-IV, 2013.
ThankYou

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Hplc (basic principles, operation and maintenance)

  • 1. HPLC ( Basic Principles, Operations and Maintenance and Troubleshooting ) Alimuzzaman Sr. Officer, R&DA Incepta pharmaceuticals Ltd, Dhaka Bangladesh Mob : 8801726041712
  • 16. Converting Normal Phase to Reverse Phase and Vice versa To convert a normal phase system/column to a reversed phase system/column, flush with a solvent that is miscible with both the current normal phase solvents and ideally Normal Phase : Hexane/Ethyl Acetate Flush : IPA then Methanol Finally : 50:50 Methanol/Water Reversed Phase : Buffered Aqueous Methanol To convert a reversed phase system/column to a normal phase system/column, follow a similar path to the one listed previously, but in reverse, for example, Reversed Phase : Buffered Aqueous Methanol Flush : 50:50 Methanol/Water Methanol then IPA Normal Phase : Hexane/Ethyl Acetate
  • 25.
  • 28.
  • 29.
  • 31.
  • 32.
  • 33.
  • 35.
  • 36.
  • 37.
  • 38.
  • 39.
  • 40. Replacement and cleaning of suction filter
  • 42. UV-VIS and PDA detector common Problem
  • 43. When to Change the Lamp
  • 44. Good Laboratory Practice for HLPC 1. Preparation of Solvents : Correct solvent preparation is very important. It can save vast amounts of time spent troubleshooting spurious peaks, base-line noise etc. 2. Quality : All reagents and solvents should be of the highest quality. HPLC grade reagents may cost slightly more than lower grade reagents, but the difference in purity is marked. HPLC grade reagents contain no impurities to produce spurious peaks in a chromatogram baseline whereas AR grade reagents do contain trace levels of impurity, which may produce spurious baseline peaks. Important: Do not store HPLC grade water in plastic containers. Additives in the plastic may leach into the water and contaminate it. Always store HPLC grade water in glass containers
  • 45. 3. Buffers : All buffers should be prepared freshly on the day required. This practice ensures that the buffer pH is unaffected by prolonged storage and that there is no microbial growth present. Changes in pH and microbial growth will affect chromatography. If buffer solutions are stored, be aware that they have a finite lifetime. Refer to pharmacopoeia monographs or similar for further guidance on buffer shelf life. Good Laboratory Practice for HLPC
  • 46.
  • 47.
  • 48. 4. Filtration : Ideally, all HPLC solvents should be filtered through a 0.45 μm filter before use. This removes any particulate matter that may cause blockages. After filtration, the solvents should be stored in a covered reservoir to prevent contamination with dust etc. Filtering HPLC solvents will benefit both your chromatography and the wear and tear of the HPLC system. Pump plungers, seals and check valves will perform better and lifetimes will be maximized. Good Laboratory Practice for HLPC
  • 49. Good Laboratory Practice for HLPC Wash Pump Injector Flow Cell Column
  • 51.
  • 52.
  • 53.
  • 54.
  • 55.
  • 56.
  • 58. References • Maintaining and trouble shooting HPLC- David J. Lunser, copyright 1981 by Wiley and sons Inc. • Modern HPLC for practicing Scientist- Micheal W. Dong. • E.L Jhonson and R. Stevenson, Basic liquid Chromatography, Varian Associates, Palo Alto, California -1978. • L.R Snyder and J. J. Kirkland, Introduction to modern Liquid Chromatography, 2nd edition. • J. K Walker M.T. Jackson Jr., and J. B. Maynard-Chromatography System- Maintenance and Trouble Shooting, 2nd edition. • Trouble Shooting in HPLC –Agilent Technologies. • Theory and Principle of HPLC –Tranining Module, Shimadzu Asia Pacific Pte Ltd, Singapore Part – I-IV, 2013.