Technical support

• Packing instruction for Kromasil in DAC columns
• Care and use of columns
• Care & Use of Kromasil Coated Chiral HPLC Columns
• Guidelines for chiral chromatography using DMB and TBB
• Optimizing your large-scale application with the software KromaGuide
• Unpacking and care of used packings
• Frequently Asked Questions

Frequently Asked Questions

Which chiral column should be used?

It is nearly impossible to foresee which chiral stationary phase will provide the highest selectivity for a certain racemate. Some common racemates that can be separated by our chiral column can be found in the application guide. If the structure of your compound is similar to the compounds shown in the application guide, then there is a good chance that the same column / mobile phase will also provide enantiomeric separation for your compound.

Kromasil AmyCoat and CelluCoat are stationary phases that are very general, thus provide separation for most racemates. These two columns can be used under normal phase, polar mode and reversed phase conditions. For reversed phase applications, specific RP columns should be used. Kromasil AmyCoat and CelluCoat are based on modified polysaccharides that are adsorbed onto a silica matrix. Attention has to be given to the choice of mobile phase solvents in order to avoid desorption of the polysaccharide polymer.

Kromasil TBB and DMB are less wide in their application, but on the other hand, they can be used with any solvent as mobile phase. Kromasil TBB shows generally good separations for acidic racemates. Kromasil DMB and TBB can be used under normal phase conditions. Best results are often obtained when an aprotic polar modifier is used, e.g. ethers or esters incombination with heptane. For basic racemates, acidic and basic additives often lead to significant improvements of the peak shape. The acidic additive (e.g. formic acid or acetic acid) should be used in excess, e.g. 0.1% acid and 0.05% amine (DEA, or TEA).

For detailed information concerning our chiral columns, please consult our chiral brochures.

Which Kromasil product corresponds to the USP column nomenclature?

USP	Description	Kromasil products
L1	Octadecyl silane chemically bonded to porous silica	Kromasil 100 Å C18 Kromasil 300 Å C18
L3	Porous silica microparticles	Kromasil 60 Å SIL Kromasil 100 Å SIL Kromasil 300 Å SIL
L7	Octyl silane chemically bonded to porous silica	Kromasil 100 Å C8 Kromasil 300 Å C8
L8	An essencially monomolecular layer of aminopropylsilane chemically bonded to totally porous silica	Kromasil 100 Å NH2
L10	Nitrile groups chemically bonded to porous silica microparticles	Kromasil 60 Å CN
L11	Phenyl groups chemically bonded to porous silica particles	Kromasil 100 Å Phenyl
L13	Trimethylsilane chemically bonded to porous silica microparticles	Kromasil 100 Å C1
L26	Butyl silane chemically bonded to totally porous silica particles	Kromasil 100 Å C4 Kromasil 300 Å C4

What is an appropriate flow rate for a certain column?

For each particle size, there is an optimal linear flow rate with respect to column efficiency, according to the van Deemter plot.

Optimal flow rate (ml/min) for Kromasil columns depending on particle size and column diameter.

	3.5 µm	5 µm	10 µm	13 µm	16 µm
Linear flow rate (cm/min)	7.1	4.7	3.3	2.4	1.9
2.1 mm ID	0.3	0.2	-	-	-
4.6 mm ID	1.5	1.0	0.7	0.5	0.4
10 mm ID	-	4.7	3.7	2.4	1.9
21.2 mm ID	-	21	15	10	8.5

For shorter separation times, the flow rate can however be increased until the pressure drop limit of the HPLC pump is reached, e.g. ca 400 bar.

How should the columns be stored?

Correct column storage is a prerequisite for problem free chromatography and a long column life time. Normal phase columns should be stored in heptane/2-propanol or another inert solvent that is free from additives.

Reversed phase stationary phases should be kept in a mixture of water / organic modifier, free from any buffers or additives that might precipitate during storage. Thus it is recommended to wash the column whenever chromatography is going to be stopped for more than 15 min with water / organic modifier 50/50, independently on whether the column will be detached from the HPLC instrument or not. If chromatography is only to be interrupted for a couple of hours it might be less laborious to keep the buffer containing mobile phase running at a very low flow rate. If the column is detached, close the inlet and outlet with a screw in order to avoid the stationary phase to dry out.

All HPLC columns should be stored at ambient temperature (18-26°C), without risk for mechanical shock, preferably in the original column box.

What is the shipping solvent?

The shipping solvent is stated on the test chromatogram and depends upon the surface modification of the stationary phase.

How can the column performance be checked?

The performance is best checked by re-running the separation shown on the enclosed test chromatogram. The exact conditions are mentioned. The sample amount should not exceed the following quantities:

Column Ø [mm ID]	test sample [µg]
2.1	2
4.6	10
10	50
21.2	225

In order to achieve representative plate counts, it is important to reduce the extra column volumes, e.g. correct tubing has to be installed between injection and the column and from the column to the detector.

How can the columns be cleaned / regenerated?

An increased back-pressure, altered retention times and loss of column performance are all symptoms of deposits in the column or on the surface of the stationary phase. Most of the times, these problems can be overcome by the use of a correctly applied washing procedure. What should also be kept in mind is that in most cases the sooner washing (regeneration) of the column is performed, the better.

Strongly adsorbed species are collected at the solvent-inlet end of the column and in many cases it is a benefit to use a reversed flow during washing. Worth mentioning is that a well packed column should not loose performance as a result of reversed flow.

RP (Hydrophobic Phases)

Deposits are most commonly present as surface adsorbed species or precipitations.

Examples of recommended solvents

Suspected Deposition/Impurity	Recommended solvents	Examples
Lipohilic	Strongly Lipophilic solvents	Al, Tol
Polar (Small peptides)	Versatile solvents	DCM, THF, DMF
Strongly Polar / Ionic (water sol.)	Aqueous solvents	50:50 DMF/w, THF/w
Polar, positively charged (amines)	Ion-exchange supressing mixtures	DMF/AA (1%), DMF/TFA (0.1%)
Macromolecular Depositions (Protein/ Large Peptide precipitations)	Strongly interaction breaking mixtures	DMF/1% SDS(aq), ACN/1% SDS(aq), Alc/AA, Alc/NEt3 (0.1%) Alc/10-100mM aqueous NaOH*
Salt/Buffer precipitations	Highly aqueous mixtures	Alc (10%)/w
	Al = Alkanes, Tol = Toluene, DCM = Dichloromethane, THF = Tetrahydrofuran, DMF = Dimethylformamide, AA = Acetic acid, TFA = Trifluoroacetic acid, ACN = Acetonitrile, Alc = Alcohol (MeOH, EtOH), w = water., NEt3 = Triethylamine, SDS = Sodiumdecylsulphate * Use as last measure for not more than 10 column volumes, also end by acidifying the phase sing Alc/1% aqueous AA 50:50.

Regeneration protocol

1. Choose solvent/solvent mixture based on impurity. If not known, assume strongly polar / ionic species in order to avoid further precipitation.
2. Use a low flow rate (10% of normal flow rate), possibly in reversed flow mode and at slightly elevated temperatures (< 40°C), for up to ten column volumes.
3. If problems with back-pressure, occasionally check progress at normal flow.
4. If the problem remains apply conditions for polar, positively charged and/or macromolecular depositions. If SDS is used, wash thoroughly with pure THF, DMF or ACN afterwards.
5. If problems persist please consult our technical support for further advice.

NP (Polar Phases)

For polar phases, especially bare silica, very strong adsorption of polar residues is common. While under normal phase conditions highly polar impurities are not eluted, however the solution to this is the use of high levels of protic solvents, possibly in combination with acid.

If there are problems with altered retention times, first check the phase - water (moisture) equilibrium. The use of dry solvents could gradually "dry" the stationary phase, resulting in altered retention times. This is especially rue for bare silica.

Regeneration protocol†

1. Eqilibrate the column using an aqueous-lipophilic mediating solvent such as THF.
2. Use a low flow rate (10% normal flow rate) of pure Alcohol (MeOH), possibly in combination with acid (Acetic acid or Formic acid, 1-5%), for up to ten column volumes.
3. If the problem persists, use a mixture of Alcohol and water, with added acid, under the same conditions as in 2.
4. As a final measure: 0.5-1.5% NH3(aq), followed by 0.5-1.5% aqueous acid (HCl, AA etc.), water, alcohol, THF and finally the actual eluent.
5. If problems persist please consult our technical support for further advice.

†: While using highly polar solvents, especially for bare silica, the stabilization of the system after washing could take a significant amount of time. This is due to the silica surface - water equilibrium being distorted.

When is a guard column recommended?

A guard column can be useful if the injection sample consists of a complex matrix with partially unknown content. However, a guard column does never make sample filtration redundant! If a guard column is to provide adequate protection for the analytical column, it must be changed often enough in order to avoid the column performance from deteriorating. By monitoring plate number (N), pressure, and resolution (Rs), the performance of the guard column, as well as the analytical column, can be assessed and a suitable moment for exchanging the guard column can be chosen.

As a rule of thumb, the guard column should be replaced when one of the following points applies:

• N decreases by > 10%
• pressure drop increases by > 10%
• Rs changes by > 10%
• more than 150 samples are injected.

When should a gradient be used?

In reverse phase HPLC it is recommended to run a scouting gradient if the conditions for a successful separation are unknown. Such a run is performed from ca 10-80% organic modifier during 30-50 min, using a linear increase in elution strength. Based on the result of this scouting gradient, either an appropriate mobile phase composition can be chosen for isocratic elution (small molecules < 1000 g/mol) or a suitable gradient for the separation of peptides or other larger molecules.

Gradient elution can also be chosen for separation of compounds that vary greatly in their polarity. As a rule of thumb, if peaks can be detected during more than 25% of the scouting gradient, gradient elution will likely be the best choice for that separation problem. If peaks appear for less than 25% of the scouting gradient, isocratic elution should be preferred, as the selectivity will always be superior under isocratic conditions.

If the sample consists of two distinct groups of compounds, step elution can lead to a good separation results. In this case one starts with isocratic mobile phase elution that renders satisfying separation results for the less retained group of compounds, followed by increasing the elution strength of the mobile phase in one step to such a degree that will separate the more retained group of compounds in an appropriate way. Step gradients can also be used for washing the column after every injection. In this case the elution strength is increased drastically after the last peak has eluted. Strongly retained impurities can then be removed from the column.

Why does the chromatogram show peak tailing?

Peak tailing can occur due to numerous reasons. The problem can be identified according to the following scheme:

• Mass overload: when injecting less sample amount (mass) either the peak becomes more symmetrical or resolves into two separate peaks.
  Corrective action: use a more dilute injection sample.
• Secondary interactions: when injecting a neutral compound (acetophenone, toluene) the peak becomes symmetrical
  Corrective action: adjust the mobile phase pH in order to render neutral analytes.

For larger ID columns (>10 mm) radial temperature gradient can also cause peak tailing. In order to avoid such, it is recommended to use a column oven. The column should be 1-2°C warmer than the mobile phase in order to compensate for the friction heat generated in the core of the column.

If neither of the above applies, the tailing can also be caused by irregularities in the column packing process or by a partially clogged inlet frit leading to an inhomogeneous flow profile.

Why does the chromatogram show poor efficiency (plate count)?

1. Injection amount / injection volume

Overloading by mass or volume as well as the wrong sample solvent can decrease the efficiency of the column significantly and therewith impair the results of the separation. The injection volume should not exceed 10% of the flow rate (e.g. 1 ml/min ⇒ injection volume < 100 µL. Mass overloading is obtained as soon as the linear part of the adsorption isotherm is surpassed. This border is individual, but as a rule of thumb, no more than 0.01 mg sample should be loaded per ml column volume (e.g. max 22 µg on 4.6 × 250 mm column). The sample mass may however be increased if necessary for detection reasons. In the sample solvent, the amount of the strong mobile phase component (alcohol, acetonitrile in RP, or alcohol, ethyl acetate etc. in NP), should not exceed the amount in the mobile phase.

2. Extra column volume / dead volumes

Poor plate counts can often be attributed to excessive dead volume. The dead volume is defined as the sum of the volume contributed by the sample injector, including the sample loop, the tubing connecting the sample injector to the column, the tubing connecting the column to the detector flow cell, the detector flow cell, plus any volume added by fittings, connectors, and in-line filters. Tubing with 0.010″ ID is commonly found in HPLC systems. If you are using narrow bore (< 3.0 mm ID) columns, or, you can enhance your system's performance by replacing the 0.010" ID tubing with 0.007″ ID tubing to reduce system dead volume. Tubing with 0.005″ ID can further reduce dead volume, but at a cost of inconvenience. Tubing with IDs less than 0.007″ restricts flow rate and may have problems with buffer salt precipitation. If you use a variety of brands of HPLC columns, make sure that the fittings used to connect to the column are properly matched. If your system has stainless steel tubing and fittings, select the proper fittings for each brand of column that you use and install those fittings prior to connecting the column. If your system has PEEK tubing and fittings, it is a good idea to install a new PEEK fitting on a freshly cut piece of PEEK tubing with each column change to insure a proper fit.

Why does the chromatogram show split peaks?

Split Peaks can be caused by:

• Column contamination
• Partially plugged frit
• Column Void
• Injection Solvent Effects
• Co-eluting compounds

Column contamination or partially clogged frits are generally caused when unfiltered samples are injected or when the sample solvent is different to the mobile phase. If the latter is the case, constituents of the sample may precipitate at the column inlet upon mixing with the mobile phase or by contact with the metallic surface of the frit.

A column void is formed either by hydrodynamic stress (high flow rate, high viscosity of the mobile phase) of a poorly packed column, by mechanical impact (the column was dropped on the floor) or by chemical dissolution of the packing material, e.g. pH > 12.

When using injection solvents that have higher elution strength than the mobile phase split or broader peaks can appear. The effect is most pronounced for early eluting peaks.

Split peaks can also occur by either two compounds that are almost co-eluting. If this is the case, the peaks should separate better if a column with higher efficiency (theoretical plates) is used. This can either be achieved by smaller particle size or a longer column. Also higher temperature and/or a less viscous mobile phase may promote a better separation.

Moreover, one compound can elute in two states, e.g. if not sufficient ion-pairing reagent is present in the mobile phase or the buffer capacity is deficient.

What can cause poorly reproducible retention times?

1. Mobile phase composition

Most reproducible results are obtained by weighing the mobile phase mixtures. For water / ethanol 30/70 (v/v) 300.0 g (300 ml x 1.0 g/ml) water are mixed with 546.0 g (700 ml x 0.78 g/ml) ethanol.

Especially when working with alcohols as polar modifier, online mixing by the HPLC pumps should be avoided, as the viscosity of the components varies significantly and hinders proper blending.

Mobile phases should always be prepared fresh, as evaporation will alter the composition of a two component mobile phase.

2. Shifting temperature

A difference of 5°C can render +/- 10% shift in retention times. It is therefore recommended to work with a column oven even when working under ambient temperature.

3. pH Control

The retention time of acidic and basic analytes depends upon the pH value. 0.1 pH unit can render a shift in retention time by 10%. It is therefore recommended to work at a pH value at least 2 pH units from the pKA.

4. Incomplete equilibration

It is recommended to equilibrate reversed phase columns with at least 10 column volumes, for buffered mobile phases with at least 20 column volumes before an analysis is initiated. Make sure all mobile phase channels are purged with the adequate mobile phase. Normal phase columns can require up to 10x longer equilibration times than reversed phase columns. Bare silica columns might take hours to equilibrate, special attention should be given to the water content in the normal phase systems. Most reproducible results are often obtained when deliberately adding 0.05% water the mobile phase.

5. Dewetting

Highly polar mobile phases can be expelled from the hydrophobic porous system, leading to less and less accessible surface area, and therewith causing shorter and shorter retention times.' see also Can the column be operated with 100% aqueous mobile phase.

Which are common buffers used in HPLC?

pH buffers

Salt	pK A	Buffer pH range	equilibrium	UV cut off
Ammonium acetate	4.76 9.2	3.8-5.8 8.2-10.2	HAc ‹—› Ac - NH 4 + ‹—› NH 3	205
Ammonium formate	3.8 9.2	2.8-4.8 8.2-10.2	HCOOH ‹—› HCOO - NH 4 + ‹—› NH 3	200
Potassium phosphate	2.1 7.2	1.1-3.1 6.2-8.2	H 3PO 4 ‹—› H 2PO 4 - H 2PO 4 - ‹—› HPO 4 2-	190
Triethylammonium acetate	4.76 11.01	3.8-5.8 10.-12.0	HAc ‹—› Ac - Et 3NH + ‹—› Et 3N	235

Additives

Salt	pK A	Buffer pH range	equilibrium	UV cut off
Acetic acid	4.76	-	HAc ‹—› Ac -	205
Formic acid	3.8	-	HCOOH ‹—› HCOO -	200
Trifluroacetic acid	0.3	-	F 3CCOOH ‹—› F 3CCOO -	210
Trietylamine	11.01	-	Et 3NH + ‹—› Et 3N	235
Diethylamine	10.5	-	Et 2NH 2 + ‹—› Et 2HN	235
Ammonium hydroxide	9.2	-	NH 4 + ‹—› NH 3	190

How should a buffered mobile phase be prepared?

Buffered mobile phases can basically be prepared in two ways:

1. preparing the buffer, including pH adjustment prior to mixing with organic modifier.
2. mixing buffer and organic modifier prior to pH adjustment.

While the pH is a well defined parameter in aqueous systems, it is not as straight forward to define or measure proton concentration in partially organic solvent systems.

It is therefore recommended to prepare the aqueous buffer, pH adjust it, filtering it through 0.4 µm and mixing it thereafter with the organic modifier. Attention should be given to the following points:

• buffers are effective within +/- 1 pH unit from their pKA ⇒ choose correct buffer system
• consider the risk of precipitation if high buffer concentrations are mixed with organic solvents
• always filter buffers through 0.4 mm filter prior to use
• be aware of the risk for bacterial or fungal growth in pure aqueous buffers
• the pH generally shifts upon the addition of an organic modifier (pH increases for inorganic buffers (e.g. phosphates) and decreases for organic buffers (e.g. acetates)
  Example: phosphate buffer pH 7.6 ⇒ addition of 40% MeOH ⇒ pH 8.5

What should be done if the back pressure is rising?

When pumping mobile phase through a particular bed, a certain pressure drop ΔP over the column will result. The relationship between particle diameter d _p and the flow velocity u is given by the Darcy's law for non-compressible solvents:

Accordingly, ΔP is proportional to the linear velocity u, the column lengths L and the viscosity of the mobile phase η, and inversely proportional to the constant k ₀ and the square of the particle diameter d _p. The constant k ₀ is a function of the interstitial porosity ε _i according to the Karman-Cozeny equation:

The equation above shows that the interstitial porosity ε _i has a tremendous influence on the permeability of the bed and therewith also on the pressure drop. For a well packed reversed phase be the interstitial porosity can be assumed to be 0.33 which leads to k ₀ = 4.45.10-4. The column permeability (d _p ²⋅k ₀) does in practice depend entirely upon the particle diameter and the particle size distribution. The latter is a very important parameter, since the particles of an HPLC packing material are never mono-disperse.

Broad distribution has two negative effects:

• a) the largest particles control the efficiency and
• b) the smallest particles control the pressure drop.

Hence, broad particle size distribution should be avoided.

What type of tubing/capillaries and connectors should be used?

Capillary tubing

When working with analytical HPLC instruments, capillaries with external diameter of 1/16″ (1.6 mm) are generally used to connect the different parts of the instrument. Those parts that do not affect the extra column volume should have internal diameters (I.D.) of 1 mm. They bring along little risk for clogging and show minimum flow resistance, which contributes to the extra column pressure drop. For those connections critical for the extra column volume, internal diameter of 0.17 mm is recommended. Such capillaries add only 23 μL extra volume per meter of tubing (1.0 mm ID tubing: 800 μL/m). In order to avoid clogging of such fine capillaries, it is of uppermost importance to filter both, mobile phases and sample solutions.

For preparative columns the tubing has to be scaled up in order to reduce the flow resistance caused by the higher flow rates (ΔP _cap≈d _cap ^-4):

Tubing sizes for column sizes

Column I.D. mm	Tubing I.D. mm
20	0.25
50	0.5
100	1.0

Fittings

Fittings are connecting the various parts of the HPLC instrument. Steel fitting usually have a separate ferrule, some designs even use two ferrules, a ring and a conical piece. When tightened the first time, the ferrule is pinched permanently and the surrounded capillary is slightly compressed. The ferrule can no longer be removed from capillary. Plastic (PEEK) fittings are one single piece (nut, ferrule), and are installed by finger tightening only. Over tightening (common with steel fittings) must be avoided, since excessive force is likely to damage the threading and the capillary. It is recommended to tighten the screw only slightly with a wrench and to test if the connection is pressure resistance, meaning, no leakage occurs once mobile phase is pumped through the system.

The distance from end of tubing to ferrule lowermost end is depends upon the column and/or instrument design. Some examples are given below:

• 0.130″ in case of Waters columns
• 0.80″ for Valco design
• 0.170″ for Rheodyne injector design

How can the column lifetime be maximized?

Column plugging is responsible for well over half of all column failures. Therefore thorough filtration (0.2 μm) of mobile phases and samples will is a key for long column lifetime.

The mobile phase compatibility is another important factor. Standard RP stationary phases are stable under pH 1.5 to 9. Under certain conditions (organic buffers) the stationary phases are even chemically stable up to pH 12. Please consult with our technical support if you would like to use your Kromasil column at pH values exceeding pH 9. Generally, organic buffers are milder towards the silica based stationary phase than inorganic ones, such as phosphates or carbonates. Further, the columns should never be left in a buffered mobile phase when the flow is interrupted for more than 10 minutes. Either choose a very low flow rate (0.1 ml/min for a 4.6 mm ID column) instead of stopping the flow completely, or exchange any buffered mobile phase with non-buffered one (e.g. water/ACN 70/30). This will prevent the column from being clogged with precipitated buffer salts.

What is "phase collapse / wettability" problem?

The use of mobile phases with a low content of organic modifier (< 5 %) generally leads to what is known as "phase collapse". The latter is best described as a dewetting phenomenon, in which the highly aqueous mobile phase is excluded from the hydrophobic pore system due to surface tension. The effect is observed predominantly with reversed phase packing materials with high ligand density (> 3.2 μmol/m ²). The loss of wetted surface results in a decrease in accessible interaction sites for the solute, and leads to a loss in retention and / or reduced loading capacity. The process can easily be reversed by purging the packed bed with a high content of organic modifier (> 50%) The phenomenon is most dominant for C18 and C8 packing materials with pores < 150 Å, but even with C4 modified packing materials, 100% aqueous mobile phases should be avoided in order to assure robust chromatography.

Can the column be operated with 100% aqueous mobile phase?

The reversed phase Kromasil columns C4, C8 and C18 should be operated with at least 5% organic modifier. Under 100% aqueous conditions, the columns are likely to undergo dewetting which means the mobile phase will be expelled from the porous system due to surface tension. In this case the analytes elute more or less with the void volume. The problem arises mainly if the flow is stopped. If a column has been dewetted, it can easily be restored by pumping mobile phase with at least 50% organic modifier through the column for ca 40 min.

Kromasil Phenyl can be used under 100% aqueous conditions without risk for dewetting.