Survey
* Your assessment is very important for improving the work of artificial intelligence, which forms the content of this project
Download Column Selection Guide
Document related concepts
no text concepts found
Transcript
01 Column Selection Guide USP-----------------------------------------------------12 Column selection guide (Biochromatography)------------------------------13 Comparison of separation mode--------- 14~16 Reversed-phase separation of peptides and proteins------------------------------------ 17~20 Column selection guide (Low molecular weight organic compounds)-----21 Application 1 (Fat-soluble vitamins, Water-soluble vitamins)--22 Application 2 (Water-soluble vitamins, Organic acids, Amino acids)---23 Reversed-phase column selection guide----24 01 Column Selection Guide Column Selection Guide USP USP CLASS No. USP Description Functional group YMC product YMC-Triart C18 YMC-Triart C18 ExRS Meteoric Core C18 Meteoric Core C18 BIO L1 Octadecyl silane chemically bonded to porous or nonporous silica or ceramic microparticles, 1.5 to 10 μm in diameter, or a monolithic silica rod. C18 page 59~61 62 72~75 YMC-UltraHT Pro C18 83 YMC-UltraHT Hydrosphere C18 83 YMC-Pack Pro C18 84 Hydrosphere C18 85 YMC-Pack Pro C18 RS 86 YMC-Pack ODS-A 87 YMC-Pack ODS-AM 87 YMC-Pack ODS-AQ 88 YMC-Pack ODS-AL 88 J'sphere ODS-H80 J'sphere ODS-M80 89 J'sphere ODS-L80 L3 Porous silica particles, 1.5 to 10 μm in diameter, or a monolithic silica rod. L7 Octylsilane chemically bonded to totally porous or superficially porous silica particles, 1.5 to 10 μm in diameter, or a monolithic silica rod. Silica YMC-Pack SIL YMC-Pack SIL-06 YMC-Triart C8 C8 104 63 Meteoric Core C8 72~75 YMC-Pack Pro C8 96 YMC-Pack C8 97 YMCbasic 100 L8 An essentially monomolecular layer of aminopropylsilane chemically bonded to totally porous silica gel support, 1.5 to 10 μm in diameter. NH2 YMC-Pack NH2 108 L10 Nitrile groups chemically bonded to porous silica particles, 1.5 to 10 μm in diameter. CN YMC-Pack CN 99 L11 Phenyl groups chemically bonded to porous silica particles, 1.5 to 10 μm in diameter. Phenyl YMC-Triart Phenyl 64 YMC-Pack Ph 98 L13 Trimethylsilane chemically bonded to porous silica particles, 3 to 10 μm in diameter. C1 YMC-Pack TMS 98 L20 Dihydroxypropane groups chemically bonded to porous silica or hybrid particles, 1.5 to 10 μm in diameter. Diol YMC-Triart Diol-HILIC 66 YMC-Pack Diol-NP 104 YMC-Pack Diol-60 YMC-Pack Diol-120 YMC-Pack Diol-200 45, 46 YMC-Pack Diol-300 12 L24 Polyvinylalcohol chemically bonded to porous silica particle, 5 μm in diameter. Polyvinylalcohol L26 Butyl silane chemically bonded to totally porous silica particles, 1.5 to 10 μm in diameter. C4 L27 Porous silica particles, 30 to 50 μm in diameter. L33 Packing having the capacity to separate dextrans by molecular size over a range of 4,000 to 500,000 Da. It is spherical, silica-based, and processed to provide pH stability. L40 Cellulose tris-3,5-dimethylphenylcarbamate coated porous silica particles, 5 to 20 μm in diameter. L43 Pentafluorophenyl groups chemically bonded to silica particles by a propyl spacer, 1.5 to 10 μm in diameter. L51 Amylose tris-3,5-dimethylphenylcarbamate-coated, porous, spherical, silica partilces, 5 to 10 μm in diameter. YMC-Pack PVA-Sil 105 YMC-Pack Pro C4 96 YMC-Pack C4 97 YMC-Pack PROTEIN-RP Silica YMC-Pack SIL-HG 99 130, 135 YMC-Pack Diol-60 Diol YMC-Pack Diol-120 YMC-Pack Diol-200 45, 46 YMC-Pack Diol-300 Cellulose tris-3,5CHIRAL ART Cellulose-C dimethylphenylcarbamate PFP YMC-Triart PFP Amylose tris-3,5CHIRAL ART Amylose-C dimethylphenylcarbamate 26~29 65 26~29 YMC-Pack Diol-60 L59 Packing for the size-exclusion separation of proteins (separation by molecular weight) over the range of 5 to 7,000 kDa. The packing is a spherical 1.5-to 10-μm, silica or hybrid packing with a hydrophilic coating. Diol L62 C30 silane bonded phase on a fully porous spherical silica, 3 to 15 μm in diameter. C30 YMC-Pack Diol-120 YMC-Pack Diol-200 45, 46 YMC-Pack Diol-300 YMC Carotenoid 100 Proteins Peptides Ion exchange Size exclusion Reversedphase Molecular weight 5,000 or less Molecular weight 5,000 or more HILIC Nucleic acids Ion exchange Oligonucleotides Nucleic acids Size exclusion Oligonucleotides Nucleic acids Reversedphase Nucleic acid bases Nucleosides Nucleotides YMC-BioPro For separation of biomolecules by the difference in surface charge P.37~39 YMC-Pack Diol For separation of biomolecules by molecular weight P.45~47 YMC-Triart C18 Meteoric Core C18 Suitable as the first choice ODS column Core-shell column with ultra fast analysis P.59~61 P.72~75 YMC-Triart C18 For separation of biomolecules with molecular weight of up to 30,000 using high temperature P.59~61 Meteoric Core C18 BIO Core-shell column for separation of biomolecules with molecular weight of up to 30,000 P.72~75 Wide-Pore Columns Column with wide pore size useful for separation of macromolecules P.17 YMC-Pack PROTEIN-RP Specialized column with excellent acid resistance for separation of proteins or peptides P.99 YMC-Triart Diol-HILIC For separation of polar compounds with poor retention on reversed-phase columns P.66 YMC-BioPro For separation of biomolecules by the difference in surface charge P.37~39 YMC-Pack Diol For separation of biomolecules by molecular weight P.45~47 YMC-Triart C18 Hydrosphere C18 Usable with 100% aqueous mobile phase P.59~61 P.83, 85 Usable with 100% aqueous mobile phase P.59~61 P.83, 85 YMC-Triart C18 Oligonucleotides Hydrosphere C18 Wide-Pore Columns HILIC Sugars Size exclusion Reversedphase HILIC Nucleic acid bases Nucleosides Nucleotides YMC-Triart Diol-HILIC YMC-Pack Polyamine II YMC-Pack Diol YMC-Triart C18 Hydrosphere C18 YMC-Triart Diol-HILIC YMC-Pack Polyamine II Column with wide pore size useful for separation of macromolecules For separation of polar compounds For separatiion or molecular weight determination of sugars Usable with 100% aqueous mobile phase For separation of polar compounds Column Selection Guide Column selection guide (Biochromatography) P.17 P.66 P.106, 107 P.45~47 P.59~61 P.83, 85 P.66 P.106, 107 13 01 Column Selection Guide Comparison of separation mode Column Selection Guide Separation of proteins by different mode Human serum Ion exchange YMC-BioPro QA 5 μm, 50 X 4.6 mmI.D. YMC-Pack Diol-300 + Diol-200 5 μm, 300 X 8.0 mmI.D. X 2 Size exclusion Albumin IgG mAU mAU Albumin Transferrin 150 Transferrin 10 100 IgG 50 0 0 N080313E 0 10 20 30 min N080616A 0 Eluent : A) 20 mM Tris-HCl (pH 8.6) B) 20 mM Tris-HCl (pH 8.6) containing 0.5 M NaCl 0-30%B (0-15 min), 30-100%B (15-30 min) Flow rate : 0.5 mL/min Temperature : 25°C Detection : UV at 280 nm Injection : 20 μL (100 μL/mL) 10 20 30 40 50 60 min Eluent : 0.1 M KH2PO4-K2HPO4 (pH 7.0) containing 0.2 M NaCl Flow rate : 0.5 mL/min Temperature : ambient (25°C) Detection : UV at 280 nm Injection : 20 μL (100 μL/mL) Proteins in human serum are separated by the difference in the surface charge on ion exchange chromatography (IEC) and by the difference in the molecular weight on size exclusion chromatography (SEC). Mouse monoclonal IgG1 anti-human IgG4 (Purified by DEAE chromatography, containing NaN3) Ion exchange Size exclusion YMC-BioPro QA-F 5 μm, 30 X 4.6 mmI.D. NaN3 YMC-Pack Diol-200 5 μm, 300 X 4.6 mmI.D. mAU mAU 4 Mouse monoclonal IgG1 (Anti-human IgG4) 40 Mouse monoclonal IgG1 (Anti-human IgG4) 5 NaN3 30 3 20 2 10 1 0 0 P080220A 0 2 4 6 8 10 12 14 16 min Eluent : A) 20 mM Tris-HCl (pH 8.1) B) 20 mM Tris-HCl (pH 8.1) containing 0.5 M NaCl 10-25%B (0-18 min) Flow rate : 1.0 mL/min Temperature : 25°C Detection : UV at 220 nm Injection : 10 μL (0.1 mg/mL) P080530A 0 5 10 15 20 25 30 min Eluent : 0.1 M KH2PO4-K2HPO4 (pH 7.0) Flow rate : 0.17 mL/min Temperature : ambient (25°C) Detection : UV at 220 nm Injection : 10 μL (0.05 mg/mL) Mouse monoclonal antibody against human IgG4 is analyzed on ion exchange chromatography (IEC) and size exclusion chromatography (SEC). Several peaks possibly derived from isoform of antibody are observed in ion exchange mode, while a single peak is detected in size exclusion mode. Mouse IgG Fc fragment (Prepared from normal serum) Size exclusion YMC-Pack Diol-200 5 μm, 300 X 8.0 mmI.D. 1. Rabbit IgG 2. Mouse IgG Fc fragment 1 50 Reversed-phase YMC-Pack C4 (300 Å) 5 μm, 150 X 4.6 mmI.D. mAU 2 mAU Mouse IgG Fc fragment 30 20 10 25 0 0 R080619B R080623D 0 5 10 15 20 min Eluent : 0.1 M KH2PO4-K2HPO4 (pH 6.9) containing 0.2 M NaCl Flow rate : 1.0 mL/min Temperature : ambient (27°C) Detection : UV at 220 nm Injection : 5 μL (0.5 mg/mL) 0 5 10 15 20 25 30 35 40 min Eluent : A) water/TFA (100/0.1) B) acetonitrile/TFA (100/0.1) 25-45%B (0-40 min) Flow rate : 1.0 mL/min Temperature : 37°C Detection : UV at 220 nm Injection : 5 μL (1.0 mg/mL) Size exclusion chromatography (SEC) is useful for separation of substances which have distinct differences in molecular weight, like between IgG and its fragments. On the other hand, reversed-phase chromatography (RPC) is suitable for a precise analysis of peptides and proteins with a molecular weight of less than 100 kDa such as IgG Fc fragment. 14 Tryptic digests of BSA Ion exchange Eluent : A) 20 mM Tris-HCl (pH 8.6) B ) 20 mM Tris-HCl (pH 8.6) containing 0.5 M NaCl 0-15%B (0-30 min), 15-60%B (30-60 min) Flow rate : 0.5 mL/min Temperature : 25°C Detection : UV at 220 nm Injection : 20 μL YMC-BioPro QA 5 μm, 50 X 4.6 mmI.D. mAU 20 10 * 0 Column Selection Guide Separation of proteins by different mode N080422B 0 Size exclusion 10 20 30 40 50 60 min Calibration curve of peptides and proteins YMC-Pack Diol-120 + Diol-60 5 μm, 500 X 8.0 mmI.D. X 2 5 10 MW mAU 60 1 4 50 10 2 40 3 103 30 4 20 10 5 * 0 Reversed-phase 10 20 30 102 101 N080623L 0 1. Myoglobin 2. Insulin (Bovine) 3. Neurotensin 4. Tetraglycine 5. Glycine 40 50 60 min (MW 17,000) (MW 5,700) (MW 1,672) (MW 246) (MW 75) Eluent : 0.1 M KH2PO4-K2HPO4 (pH 7.0) containing 0.2 M NaCl/acetonitrile (70/30) Flow rate : 0.7 mL/min Temperature : ambient (25°C) Detection : UV at 220 nm Injection : 5 μL YMCbasic 5 μm, 150 X 2.0 mmI.D. mAU 40 30 * 20 10 0 N080318B 0 10 20 30 40 50 60 min * undigested BSA Eluent : A) water/TFA (100/0.1) B) acetonitrile/TFA (100/0.1) 5-35%B (0-50 min), 35-45%B (50-55 min), 45%B (55-60 min) Flow rate : 0.2 mL/min Temperature : 37°C Detection : UV at 220 nm Injection : 1 μL These chromatograms show separation of tryptic digests of BSA (MW: 66,000) in ion exchange chromatography (IEC), size exclusion chromatography (SEC) and reversed-phase chromatography (RPC). The molecular weight of the digests is estimated to be approximately from 100 to 20,000 by SEC chromatogram. IEC and RPC chromatograms show many peaks of fragments which are separated by the difference in structure, charge and hydrophobicity. Separation of sugar chains by different mode Pyridylamino (PA) -Sugar chains Reversed-phase YMC-Pack ODS-A (120 Å) 5 μm, 150 X 4.6 mmI.D. Normal-phase 1.PA-Sugar Chain 014 YMC-Pack Polyamine II 5 μm, 150 X 4.6 mmI.D. 2.PA-Sugar Chain 001 3.PA-Sugar Chain 002 0 10 20 min G910607A Eluent : methanol/20 mM NH4H2PO4 (5/95) Flow rate : 1.0 mL/min Temperature : 37°C Detection : FLS at Ex. 320 nm, Em. 400 nm Injection : 2 μL (3.3 pmol/mL) Sample : PA-Sugar Chain Series, manufactured by TAKARA BIO INC. 0 10 20 min G910620A Eluent : methanol/20 mM NH4H2PO4 (80/20) Flow rate : 1.0 mL/min Temperature : 37°C Detection : FLS at Ex. 320 nm, Em. 400 nm Injection : 3 μL (3.3 pmol/mL) Sample : PA-Sugar Chain Series, manufactured by TAKARA BIO INC. Pyridylamino (PA) sugar chains are often analyzed for structural determination of sugar chain in glycoproteins and glycolipids. Separations of PA sugar chains in reversed-phase (RP) mode and normal-phase (NP) mode are shown. Two dimensional HPLC combining two different modes, such as RP mode and NP mode, is useful tool for structural determination of sugar chain. 15 01 Column Selection Guide Comparison of separation mode Column Selection Guide Separation of nucleic acids by different mode DNA fragments 1 Kb DNA ladder (75 - 12,216 bp) Ion exchange Eluent : A) 20 mM Tris-HCl (pH 8.1) containing 0.7 M NaCl B ) 20 mM Tris-HCl (pH 8.1) containing 1.0 M NaCl 0-100%B (0-30 min) Flow rate : 0.5 mL/min Temperature : 25°C Detection : UV at 260 nm Injection : 20 μL YMC-BioPro QA-F 5 μm, 100 X 4.6 mmI.D. mAU 100 50 0 N080212G 0 10 20 30 min DNA fragments are analyzed with YMC-BioPro QA-F ion exchange column. 100 mm length column of YMC-BioPro QA-F is ideal for high-resolution analysis of nucleic acids. Plasmid pBR322 restriction fragments Ion exchange Eluent YMC-BioPro QA-F 5 μm, 100 X 4.6 mmI.D. Plasmid pBR322 Hae III digests (8-587 bp) mAU 40 Plasmid pBR322 (4,361 bp) 30 : A) 20 mM Tris-HCl (pH 8.1) B ) 20 mM Tris-HCl (pH 8.1) containing 1.0 M NaCl 70-85%B (0-20 min), 85%B (20-25 min) Flow rate : 0.5 mL/min Temperature : 35°C Detection : UV at 260 nm Injection : 10 μL 20 10 0 N080610F 0 5 Size exclusion 10 15 20 25 min YMC-Pack Diol-300 + Diol-200 5 μm, 500 X 8.0 mmI.D. X 2 Plasmid pBR322 Hae III digests (8-587 bp) mAU Plasmid pBR322 (4,361 bp) 40 30 Eluent 20 10 0 P080617A 0 10 20 30 40 50 min :0 .1 M KH2PO4-K2HPO4 (pH 7.0) containing 0.2 M NaCl Flow rate : 0.7 mL/min Temperature : ambient (25°C) Detection : UV at 260 nm Injection : 10 μL The separation of plasmid pBR322 restriction fragments (8-857 bp) is compared between in ion exchange mode and size exclusion mode. Ion exchange chromatography (IEC) is applicable to identification of each fragment requiring high resolution and size exclusion chromatography (SEC) is usable for characterization of molecular weight distribution. Oligonucleotide (mi RNA) YMC-Triart C18 3 μm, 150 X 2.0 mmI.D. 5’-pUGG AGU GUG ACA AUG GUG UUG-3’ 5’-pUGG AGU GUG ACA AUG GUG UUG U-3’ UV mAU 20 (21 nt, MW 6890.1) (22 nt, MW 7196.3) 21 nt 22 nt 10 0 0.0 MS 2.5 5.0 7.5 5 10.0 12.5 15.0 21 nt 0 0.0 17.5 min MIC (m/z 1721.5, m/z 1798.1) 2.5 5.0 7.5 10.0 12.5 15.0 22 nt 17.5 min Courtesy of M.Yamada, SHIMADZU CORPORATION 16 Eluent : A) 10 mM DBAA* (pH 7.5) B) 10 mM DBAA* (pH 7.5)/acetonitrile (50/50) 62-72%B (0-20 min) Flow rate : 0.2 mL/min Temperature : 30°C Detection : UV at 260 nm and ESI-negative mode Injection : 4 μL (5 nmol/mL) Instrument : LC) Shimadzu Prominence MS) Shimadzu LCMS2020 * di-n-butylamine-acetic acid This figure shows LC/MS analysis of oligonucleotides in reversed-phase mode. YMC-Triart C18 columns are useful for oligonucleotides and they can achieve excellent separation by onenucleotide difference and sufficient intensity in UV and ESI-MS. Reversed-phase separation of peptides and proteins Functional group Molecular weight of sample C18 C8 C4 Pore size 120 Å 5,000 200 Å Column Selection Guide How to select reversed-phase columns To separate proteins or peptides, it is important to select columns based on the molecular weight of the compounds to be separated. As shown in the table on the right, the C18 column with 120 Å pore size is generally suitable for small peptides up to MW 5,000. In the case of large peptides or small proteins up to MW 20,000, the C8 column with 200 Å pore size often gives the best column efficiency. Furthermore, most of proteins are eluted effectively by the C4 column with 300 Å. Separation may also be influenced by the hydrophobicity of the analyte and the type of the functional group as well as molecular weight. If the sufficient separation is not achieved with columns marked with a double circle, perform optimization as indicated by the arrows shown in the table. In addition to columns C18, C8, and C4 shown in the table, PROTEIN-RP and CN type columns with different selectivity are also useful. 20,000 300 Å 100,000 Separation of peptides (MW 574 - 3,465) Excellent peak shapes for basic peptides Hydrosphere C18 (120 Å) 5 μm, 150 X 4.6 mmI.D. 1 4 2 6 5 3 4 5 23 7 6 1 5 10 15 A000313D 20 min 0 5 10 15 (MW 1,425) (MW 587) (MW 1,746) (MW 574) (MW 588) (MW 1,899) (MW 3,465) Eluent : A) water/TFA (100/0.1) B) acetonitrile/TFA (100/0.1) 20-40%B (0-15 min), 40%B (15-20 min) Flow rate : 1.0 mL/min Temperature : 37°C Detection : UV at 220 nm 7 A000308B 0 1. BAM-12P 2. [D-Ala2,Met5]-Enkephalinamide 3. α-Endorphin 4. Met-Enkephalin 5. [D-Ala2,Met5]-Enkephalin 6. γ-Endorphin 7. β-Endorphin Brand E2 (100 Å) 5 μm, 150 X 4.6 mmI.D. (ODS column for hydrophilic compounds) 20 min Generally, the conventional C18 column with 120 Å pore size is suitable for analysis of small peptides up to 5,000 in molecular weight. Especially Triart and Pro series ODS columns, which are processed with advanced endcapping technology, are ideal for separation of basic peptides. As shown in the above, Hydrosphere C18, a Pro series column, exhibits excellent separations and superior peak shapes of basic peptides (peak 1 and 7), in contrast to the commercial ODS column for hydrophilic compounds, Brand E2. Separation of peptides and proteins (MW 4,300 - 17,000) Comparison of separation on columns with different pore size and functional group Pore size C8, 120 Å 1 2 Functional group 1 C18, 200 Å 4 5 3 2 6 4 3 5 6 04072910.D 04073006.D 1 C8, 300 Å 4 2 1,2 C4, 200 Å 6 4 6 5 3 3 5 10 15 04080204.D 04073002.D 0 5 10 15 min 0 5 1. Cytochrome c 2. Insulin (Bovine) 3. Amyloid β-protein 4. Lysozyme 5. α-Lactalbumin 6. Myoglobin Optimized combination of pore size and functional group C8, 200 Å 1 6 4 2 5 3 04082002.D 0 5 10 15 min min (MW 12,400) (MW 5,700) (MW 4,300) (MW 14,300) (MW 14,100) (MW 17,000) Column : 5 μm, 150 X 4.6 mmI.D. Eluent : A) water/TFA (100/0.1) B) acetonitrile/TFA (100/0.1) 25-60%B (0-20 min) Flow rate : 1.0 mL/min Temperature : 37°C Detection : UV at 220 nm For proteins and peptides with molecular weight of 4,300 to 17,000, separation characteristics are compared using columns with different pore size and functional group. In accordance with the table above, the suitable column is C8, 200 Å for groups of compounds with a molecular weight within this range. If either pore size or functional group of the packing material is not optimized, peak broadening and poor resolution are observed. By using the most suitable column (C8, 200 Å) for the target compounds, sharp peak shapes and excellent separation are achieved. 17 01 Column Selection Guide Reversed-phase separation of peptides and proteins Column Selection Guide Separation of proteins (MW 66,000 - 96,000) Optimization of eluent conditions (C4, 300 Å) 1 1 1. BSA (MW 66,000) 2. Conalbumin (MW 77,000) 3. Lipoxidase (MW 96,000) 2 2 2-propanol addition 3 3 05011405.D 0 5 10 15 Column : YMC-Pack C4 (5 μm, 300 Å) 150 X 4.6 mmI.D. Gradient : 30-75%B (0-15 min), 75%B (15-20 min) Flow rate : 1.0 mL/min Temperature : 37°C Detection : UV at 220 nm 04093007.D min 0 5 10 15 min A)water/TFA (100/0.1) B)acetonitrile/2-propanol/TFA (50/50/0.1) A)water/TFA (100/0.1) B)acetonitrile/TFA (100/0.1) Gradient elution of water and acetonitrile containing TFA are often employed in an analysis of proteins and peptides. In some cases, addition of a “third solvent” is effective for change in selectivity and separation. The above example shows the resolution between highmolecular weight proteins (peak 1 and 2) is improved by adding 2-propanol into the standard mobile phase of acetonitrile/water/TFA. Comparison of separation on columns with different pore size and functional group 1 1. BSA (MW 66,000) 2. Conalbumin (MW 77,000) 3. Lipoxidase (MW 96,000) C4, 300 Å Column Eluent : 5 μm, 150 X 4.6 mmI.D. : A) water/TFA (100/0.1) B ) acetonitrile/2-propanol/TFA (50/50/0.1) 30-75%B (0-15 min), 75%B (15-20 min) Flow rate : 1.0 mL/min Temperature : 37°C Detection : UV at 220 nm 2 3 04093007.D 0 4 8 12 16 min Pore size Functional group 1 C4, 200 Å 12 2 3 C8, 300 Å 3 05011711.D 05011708.D C4, 120 Å 1 2 12 3 C18, 300 Å 3 05011714.D 0 4 8 12 16 min 05011802.D 0 4 8 12 16 min Separation characteristics of proteins with molecular weight of 66,000 to 96,000 are compared using columns with different pore size and functional group. The columns with smaller pore size, which have the same C4 functional groups, provide broader peak shapes and poor separations. In comparison among the 300 Å pore columns with different functional groups, the longer alkyl chain such as C18 and C8 results in poor resolution. It is important to choose optimal pore size and functional group depending on molecular weight of proteins for better peak shapes and resolutions. Proteins with molecular weight of 20,000 to 100,000 are separated effectively by the C4 column with 300 Å pore size. 18 Column Selection Guide Effect of column temperature on separation of peptides and proteins Condition A (MW 500-18,400) mAU 60 21.8-25.8 MPa (3,160-3,740 psi) 50 40˚C 1 Condition B (MW 14,300-25,700) mAU Peak capacity = 230 60 2 50 40 37.0-37.5 MPa (5,370-5,440 psi) 1 2 40 4, 3 30 3 30 5 20 20 10 10 0 F111228B 0.0 0.5 1.0 1.5 2.0 mAU 60 2.5 1 15.8-18.5 MPa (2,290-2,680 psi) 50 70˚C Peak capacity = 67 3.0 3.5 0 min* F111226B 0.0 0.5 1.0 1.5 2.0 mAU Peak capacity 2 = 279 60 50 40 3.0 3 4 min* 3 30 5 20 4.0 2 40 30 3.5 Peak capacity = 107 1 27.4-28.4 MPa (3,970-4,120 psi) 2.5 20 10 10 0 F111228A 0.0 0.5 Analytes Condition A 1. Oxytocin 2. Leu-Enkephalin 3. β-Endorphin 4. Insulin 5. β-Lactoglobulin A Condition B 1. Lysozyme 2. α-Chymotrypsinogen 3. β-Lactoglobulin A 1.0 1.5 2.0 2.5 MW Peak width ½(min ) 40°C 70°C 1,007 0.017 0.014 556 3,465 5,733 18,400 0.015 0.043 0.015 0.016 0.015 0.030 14,300 25,700 18,400 0.069 0.080 0.080 0.044 0.049 0.048 3.0 3.5 min* Column Eluent Gradient Flow rate Detection Injection System 0 F111226A 0.0 0.5 1.0 1.5 2.0 2.5 3.0 3.5 4.0 min* : YMC-Triart C18 (1.9 μm, 120 Å) , 50 X 2.0 mmI.D. : A) water/TFA (100/0.1) B) acetonitrile/TFA (100/0.1) - condition A B) acetonitrile/2-propanol/TFA (50/50/0.1) - condition B : 10-80%B (0-5 min) - condition A 30-60%B (0-5 min) - condition B : 0.4 mL/min : UV at 220 nm : 1 μL (50 μg/mL) - condition A 1 μL (250 μg/mL) - condition B : Agilent 1200SL PC (peak capacity) = 1 + (gradient time/peak width*) *peak width = 2W0.5h average The effect of temperature on separation of peptides and proteins with a variety of molecular weight (MW) is estimated. The separations at 40°C and 70°C are compared. By increasing column temperature to 70°C, selectivity change is observed, and peaks become sharper. Thus, improved resolution especially for larger molecules is obtained. Generally, larger molecules diffuse very slowly compared to small molecules. An elevated temperature can improve efficiency and peak shape by lowering mobile phase viscosity and improving mass transfer. Temperature is a simple and effective tool to increase resolution in separation of proteins and peptides. 19 01 Column Selection Guide Reversed-phase separation of peptides and proteins Column Selection Guide Improvement of resolution by increasing column temperature and coupling of 1.9 μm columns Peak capacity = 365 40˚C 1.9 µm, 100 X 2.0 mmI.D. 15 min gradient 46.5-48.5 MPa (6,740-7,030 psi) mAU 30 20 10 0 P110705A 0 70˚C 2 4 6 8 10 12 Peak capacity = 450 30 27.6-28.6 MPa (4,000-4,150 psi) 20 10 Coupling of two columns 9 0 58.1-61.6 MPa (8,430-8,930 psi) 2 4 6 8 10 12 10.2 10.6 min 14 15 min 30 20 10 19 20 21 min P110707A 0 20 9.8 25mAU Peak capacity = 630 0 Column Eluent Flow rate Detection Injection Sample System 9.4 P110728A 0 mAU Two coupled 1.9 µm, 100 X 2.0 mmI.D. 30 min gradient min 25mAU mAU 1.9 µm, 100 X 2.0 mmI.D. 15 min gradient 15 14 : YMC-Triart C18 (1.9 μm, 120 Å) : A) water/TFA (100/0.1) B) acetonitrile/TFA (100/0.08) 5-40%B (0-15 min) for a single column 5-40%B (0-30 min) for two coupled columns : 0.4 mL/min : UV at 220 nm : 10 μL for a single column 20 μL for two coupled columns : Tryptic digest of Bovine Hemoglobin : Agilent 1290 4 8 12 16 20 24 28 30 min 23% more peaks can be resolved by increasing the column temperature to 70°C in the separation of tryptic digest of Hemoglobin. The outstanding efficiency obtained by a coupling of two 100 mm length of Triart 1.9 μm columns reduces co-elution peaks and allows the precise separation in an analysis of complicated samples, such as peptide mapping. Pharmaceutical products Reversedphase YMC-Triart C18 YMC-Triart (C18, C18 ExRS, C8, PFP, Phenyl) Effective for method screening with 5 chemistries Agricultural chemicals Metabolites Suitable as the first choice column for reversed-phase separation P.59~61 P.59~65 Normalphase YMC-Pack SIL, SIL-06 Standard normal-phase column P.104 YMC-Pack Diol-NP Normal-phase column providing separation characteristics different from bare silica gel P.104 Others HILIC YMC-Triart Diol-HILIC For separation of polar compounds with poor retention on reversed-phase columns Vitamins Reversedphase Food additives Natural products Water-soluble vitamins Fat-soluble vitamins HILIC Normalphase Organic acids Fatty acids Water-soluble vitamins Fat-soluble vitamins Reversedphase Normalphase Phospholipids Reversedphase YMC-Triart C18 P.59~61 P.59~61 YMC Carotenoid (C30) YMC-Pack Polyamine II, NH2 For separation of water-soluble vitamins such as P.106~108 vitamin C under HILIC mode YMC-Triart Diol-HILIC For simultaneous separation of water-soluble vitamins YMC-Pack SIL, SIL-06 For separation of fat-soluble vitamins such as tocopherol YMC-Pack ODS-AL YMC-Pack Polyamine II YMC-Triart C18 Usable with 100% aqueous mobile phase YMC-Pack SIL, SIL-06 Standard normal-phase column YMC-Triart C18 For separation of molecular species P.88 P.100 P.66 P.104 P.106, 107 P.59~61 P.104 P.59~61 For separation of phospholipid classes P.104, 105 YMC-Pack Diol-NP HILIC Free amino acids Reversedphase Free amino acids YMC-Triart Diol-HILIC For simultaneous separation of amino acids under HILIC mode YMC-Triart C18 Usable with 100% aqueous mobile phase Hydrosphere C18 For separation of hydrophobic amino acids P.59~61 P.83, 85 YMC-Triart C18 Suitable as the first choice ODS column P.59~61 P.66 Reversedphase YMC Carotenoid (C30) YMC-Triart C8 YMC-Triart PFP CHIRAL ART High-density bonding for excellent ability to recognize planar structure For carotenoids separation For separations of isomers or structural analogs For separations of polar compounds or isomers For separations of isomers or structural analogs Normalphase YMC-Pack SIL, SIL-06 Standard normal-phase column CHIRAL ART For separations of isomers or structural analogs P.26~29 Reversedphase CHIRAL ART YMC CHIRAL NEA For separation of optical isomers P.26~30 Normalphase CHIRAL ART For separation of optical isomers P.26~30 YMC-Triart C18 ExRS Optical isomers (For separation under a buffered or ion pairing mobile phase) Suitable as the first choice ODS column Non-endcapped ODS, suitable for separation of compounds with similar structure Separation behavior different from ODS YMC-Pack PVA-Sil Labeled amino acids Structural isomers Usable with 100% aqueous mobile phase P.66 YMC-Pack SIL, SIL-06 Normalphase Amino acids YMC-Triart C18 Column Selection Guide Column selection guide (Low molecular weight organic compounds) YMC CHIRAL NEA P.62 P.100 P.63 P.65 P.26~29 P.104 21 01 Column Selection Guide Application 1 (Fat-soluble vitamins, Water-soluble vitamins) Column Selection Guide Vitamin D Reversed-phase Vitamin E (Tocopherols) Normal-phase Separation of structurally similar compounds Separation of tocopherol homologues 1. mAU H H 1. CH3 H3C CH3 CH3 H 15 CH3 CH3 O CH3 HO 3 1 H3C α-Tocopherol CH3 CH3 4 CH3 2. CH3 HO 1 10 HO 3. H 2 Ergocalciferol (Vitamin D2) 4. CH3 H 5 CH3 CH3 CH3 CH3 CH3 CH3 CH3 CH3 CH3 CH3 CH3 O CH3 HO 2 H H3C CH3 2. H3C CH3 β-Tocopherol CH3 CH2 CH3 CH3 CH3 O H CH3 γ-Tocopherol CH3 CH3 O CH3 HO δ-Tocopherol H CH2 HO 0 H Cholecalciferol (Vitamin D3) 0 10 20 30 min (P040819C) Column : YMC-Pack ODS-AL (5 μm, 120 Å) 150 X 4.6 mmI.D. Eluent : acetonitrile/water (95/5) Flow rate : 1.0 mL/min Temperature : 40°C Detection : UV at 265 nm Injection : 10 μL (0.01 mg/mL) Reversed-phase 0 5 10 15 min (S970702A) Column : YMC-Pack SIL (5 μm, 120 Å) 250 X 4.6 mm I.D. Eluent : n-hexane/2-propanol/acetic acid (1000/6/5) Flow rate : 1.4 mL/min Temperature : 35°C Detection : FLS at Ex 298 nm, Em 325 nm Injection : 20 μL (5~20 μg/mL) Water-soluble vitamins Water-soluble vitamins HILIC Simultaneous separation of water-soluble vitamins under ion pairing mobile phase Simultaneous separation of water-soluble vitamins under HILIC mode O 1. mAU 1 3 20 5 15 O O OH NH2 N N Nicotinic acid Nicotinamide 9. 4 3. • HCl 4. OH OH 2-O-α-D-Glucopyranosyl -L-ascorbic acid (Ascorbic acid 2-glucoside) NH N O 10. 10 6 N OH 5. 0 5 10 15 20 25 4 6 8 10 12 14 16 18 20 min* min Column : YMC-Triart C18 (5 μm, 120 Å) 250 X 4.6 mmI.D. Eluent : phosphate buffer*/acetonitrile (90/10) *Dissolve 1.4 g KH2PO4 in 800 mL water → add 26 mL 10% TBA·OH → adjust pH 5.2 by 20% H3PO4 → add water to make 1000 mL Flow rate : 0.8 mL/min Temperature : 40°C Detection : UV at 260 nm Injection : 10 μL (5 μg/mL) 22 11. O O H2 N H 2N NH2 N Orotic acid O CN N + Co N O N NH2 6. HO HO H O O N H O OH Erythorbic acid (D-Isoascorbic acid) O O O NH2 N O P (F121012A) O O H2 N HO (R100315D) - Cl • HCl NH N H O 2 OH S O HO 0 + Thiamine hydrochloride 0 0 N N Riboflavin 3 4 NH2 OH HO 50 O HO O N OH O O N 78 O OH N 12 5 H HO Pyridoxine hydrochloride 11 5 HO HO OH OH OH 100 9 O OH L-Ascorbic acid 8. 2. 6 7 H O HO Caffein 150 10 HO HO N N 9 2 N O mAU 8 7. N 1. Thiamine HCl (Vitamin B1) 2. Pyridoxine HCl (Vitamin B6) 3. Nicotinamide 4. Cyanocobalamin (Vitamin B12) 5. L-Ascorbic acid 2-glucoside 6. L-Ascorbic acid (Vitamin C) 7. Erythorbic acid 8. Riboflavin (Vitamin B2) 9. Nicotinic acid O HO N - HO O Cyanocobalamin Column : YMC-Triart Diol-HILIC (5 μm, 120 Å) 150 X 3.0 mmI.D. Eluent : A) acetonitrile/200 mM HCOOH-HCOONH4 (pH 3.6)/water (90/5/5) B) acetonitrile/200 mM HCOOH-HCOONH4 (pH 3.6)/water (50/5/45) 0-75%B (0-20 min) Flow rate : 0.425 mL/min Temperature : 40°C Detection : UV at 254 nm Injection : 4 μL (50 μg/mL) Application 2 (Water-soluble vitamins, Organic acids, Amino acids) Organic acids Reversed-phase Separation of ascorbic acid under HILIC mode Simultaneous separation of organic acids under 100% aqueous mobile phase 1. Oxalic acid 2. Tartaric acid 1. Nicotinic acid 2. Erythorbic acid 3. L-Ascorbic acid 1 3. Glycolic acid mAU 2,3 4. Formic acid 50 5. L-Malic acid 6. Malonic acid 7. Lactic acid 12 40 2 3 8. Acetic acid 4 9. Maleic acid 13 30 1 Column Selection Guide Vitamin C (Ascorbic acid) HILIC 10. Citric acid 11. Succinic acid 56 8 12. Fumaric acid 9 10 20 13. Acrylic acid 11 14. Propionic acid 14 7 10 0 10 20 0 min 0 2 4 6 8 min 10 (A970603A) Column : YMC-Pack Polyamine II 250 X 4.6 mmI.D. Eluent : acetonitrile/50 mM NH4H2PO4 (70/30) Flow rate : 1.0 mL/min Temperature : 30°C Detection : UV at 250 nm, 0.16 AUFS Injection : 10 μL (0.05~0.1 mg/mL) HILIC (U111212Q) Column : YMC-Triart C18 (3 μm, 120 Å) 150 X 3.0 mmI.D. Eluent : 20 mM phosphoric acid Flow rate : 0.425 mL/min Temperature : 37°C Detection : UV at 220 nm Injection : 2 μL (0.005~1.5 mg/mL) Amino acids Amino acids Reversed-phase Simultaneous separation of amino acids under HILIC mode Separation of hydrophobic amino acids under highly aqueous mobile phase (JP method) pA 500 Standard solution* 1 * (1.10 mg/mL L-Valine, 0.92 mg/mL L-Isoleucine, 1.84 mg/mL L-Leucine) Phenylalanine (Phe) Tryptophan (Trp) 400 mAU Leucine (Leu) Methionine (Met) Tyrosine (Tyr) * 3 1 Isoleucine (Ile) ** 150 Valine (Val) 300 Cysteine HCl (Cys) Proline (Pro) 2 100 System suitability requirement Threonine (Thr) Resolution (2, 3) γ-Aminobutyric acid (GABA) 200 Serine (Ser) 2.68 1 Relative standard deviation of the retention time (each of the peaks) 50 Result 1.5 Alanine (Ala) 1.0% Glycine (Gly) 0.02% 2 0.02% 3 0.02% Asparagine (Asn) Glutamine (Gln) Citrulline (Cit) 100 Glutamic acid (Glu) Histidine (His) * Aspartic acid (Asp) Lysine (Lys) 0 Ornithine HCl (Orn) 2.0 4.0 0 2 6.0 8.0 10.0 12.0 14.0 16.0 18.0 min *Chloride ion contained in the sample solution **Sodium ion contained in the sample solution (F130618A) 4 1. 6 2. H COOH H3C H NH2 L-Valine min 3. CH3 Arginine HCl (Arg) * 0.0 0 CH3 COOH H3C COOH H3C H NH2 L-Isoleucine H3C H NH2 L-Leucine (U120210A) Column : YMC-Triart Diol-HILIC (5 μm, 120 Å) 150 X 4.6 mmI.D. Eluent : A) 100 mM HCOOH-HCOONH4 (pH 3.6) B) acetonitrile 83-80%B (0-12 min), 80-68%B (12-20 min) Flow rate : 1.0 mL/min Temperature : 40°C Detection : Corona® CAD® (Charged Aerosol Detector) Injection : 10 μL (0.1 mg/mL) Column : YMC-Triart C18 (3 μm, 120 Å) 150 X 4.6 mmI.D. Eluent : phosphate buffer (pH 2.8)*2/acetonitrile (97/3) *2 Dissolve 31.2 g of NaH2PO4·2H2O in 1000 mL of water and adjust pH 2.8 with H3PO4 Flow rate : 0.9 mL/min (adjust the flow rate so that the retention time of L-Valine is about 2.5 min) Temperature : 40°C Detection : UV at 210 nm Injection : 20 μL (The Japanese Pharmacopoeia 16th; Identification) Corona and CAD are trademarks of Thermo Fisher Scientific. *1 Standard solution was prepared from L-Valine, L-Isoleucine and L-Leucine supplied as a reagent for laboratory use. 23 01 Column Selection Guide Reversed-phase column selection guide 2nd choice! Versatile column for separation of both hydrophilic and hydrophobic compounds Similar structures (Isomers) Improvement of resolution Column Selection Guide 1st choice! Triart C18 Triart C18 ExRS Triart C8 YMC-Pack ODS-AL YMC Carotenoid Optical Isomer Separation Columns Aromatic compounds (π-electron acceptor ) Conjugated compounds Triart Phenyl Aromatic compounds (π-electron donor) Cis-trans isomers Polar compounds Halogenated compounds With typical structure or functional group Effective for separation of compounds with difficulty on other C18 column!! • Only weak retention • Poor peak shape • pH limit for mobile phase etc. Triart PFP Improvement of retention Mobile phase Change Temperature Too much retention/resolution (Long run time) Triart C8 Basic compounds Weak retention (Highly polar compounds) Triart PFP HILIC mode (Triart Diol-HILIC) Comparison of hydrophobicity and hydrogen-bonding capacity of various columns 0.170 Hydrophilic ODS Hydrophobicity: Low Pro C4 Hydrogen-bonding capacity: High Hydrogen binding capacity [α(Caffeine/Benzene)] 0.150 Develosil C30-UG Atlantis dC18 Hydrosphere C18 ZORBAX SB-C18 Atlantis T3 0.130 CAPCELL PAK C18 AQ TSKgel ODS-80Ts Develosil ODS-MG Standard ODS column CAPCELL PAK C18 MGIII Pro C8 0.110 Gemini C18 Pro C18 Unison UK-C18 Gemini-NX C18 0.070 Hydrogen-bonding capacity: Moderate CAPCELL PAK C18 MGII Hypersil GOLD 0.090 Hydrophobicity: Moderate CAPCELL PAK C18 MG Inertsil ODS-4 XTerra MS C18 Meteoric Triart C8 Core C8 Sunfire C18 Luna C18(2) Inertsil ODS-3 XBridge C18 Mightysil RP-18 Eternity-C18 L-column ODS Develosil ODS-SR Triart C18 Symmetry C18 TSKgel ODS-100S Cadenza CD-C18 L-column2 ODS Hydrophobic ODS Hydrophobicity: High Hydrogen-bonding capacity: Low ZORBAX Extend-C18 Meteoric Core C18 CAPCELL PAK C18 ACR Pro C18 RS InertSustain C18 0.050 Triart C18 ExRS Eluent: methanol/water (80/20) [Amylbenzene] methanol/water (30/70) [Caffeine, Benzene] (S150318A) 0.030 1.00 3.00 5.00 7.00 9.00 11.00 Hydrophobicity [k’(Amylbenzene)] 24 13.00 15.00 17.00
Related documents