Apparatus and method for preparative supercritical fluid chromatography

BACKGROUND OF THE INVENTION

A substantial need exists for industries to recover purified components of interest from samples containing simple or complex mixtures of components. Many technologies have been developed to meet this need. For dissolvable, nonvolatile components, the technology of choice has been liquid elution chromatography.

Analysts have several objectives in employing preparative elution chromatography. First, they wish to achieve the highest available purity of each component of interest. Second, they wish to recover the maximum amount of the components of interest. Third, they wish to process sequential, possibly unrelated samples as quickly as possible and without contamination from prior samples. Finally, it is frequently desirable to recover samples in a form that is rapidly convertible either to the pure, solvent-free component or to a solution of known composition which may or may not include the original collection solvent.

In the case of normal phase chromatography, where only organic solvents or mixtures are used as eluants, typical fraction volumes of tens to hundreds of milliliters are common. The fraction must then be evaporated over substantial time to recover the component residues of interest. In reversed phase chromatography, where mixtures of organic solvents and water are used as the elution mobile phase, a secondary problem arises. After removal of lower boiling solvents, recovered fractions must undergo a water removal step lasting from overnight to several days. Thus, availability of the recovered components of interest is delayed by hours or days, even after the separation process is complete. This latter problem can create a serious bottleneck in the entire purification process when enough samples are queued.

Where difficult separation conditions exist or separation speed is a requirement, a subset of elution chromatography, known as high performance liquid chromatography (HPLC), is preferred. This HPLC technique is used both as an analytical means to identify individual components and as a preparative means of purifying and collecting these components.

For analytical HPLC, samples with component levels in the nanogram to microgram range are typical. Preparative HPLC systems typically deal with microgram to multiple gram quantities of components per separation. Preparative HPLC systems also require a means to collect and store individual fractions. This is commonly performed, either manually or automatically, simply by diverting the system flow stream to a series of open containers.

Drawbacks exist to the current use of preparative HPLC. Elution periods ranging from several minutes to hours are necessary for each sample. Further, even in optimal conditions only a small fraction of the mobile phase contains components of interest. This can lead to very large volumes of waste mobile phase being generated in normal operation of the system.

An alternative separation technology called supercritical fluid chromatography (SFC) has advanced over the past decade. SFC uses highly compressible mobile phases, which typically employ carbon dioxide (CO2) as a principle component. In addition to CO2, the mobile phase frequently contains an organic solvent modifier, which adjusts the polarity of the mobile phase for optimum chromatographic performance. Since different components of a sample may require different levels of organic modifier to elute rapidly, a common technique is to continuously vary the mobile phase composition by linearly increasing the organic modifier content. This technique is called gradient elution.

SFC has been proven to have superior speed and resolving power compared to traditional HPLC for analytical applications. This results from the dramatically improved diffusion rates of solutes in SFC mobile phases compared to HPLC mobile phases. Separations have been accomplished as much as an order of magnitude faster using SFC instruments compared to HPLC instruments using the same chromatographic column. A key factor to optimizing SFC separations is the ability to independently control flow, density and composition of the mobile phase over the course of the separation.

SFC instruments used with gradient elution also reequillibrate much more rapidly than corresponding HPLC systems. As a result, they are ready for processing the next sample after a shorter period of time. A common gradient range for gradient SFC methods might occur in the range of 2% to 60% composition of the organic modifier.

It is worth noting that SFC instruments, while designed to operate in regions of temperature and pressure above the critical point of CO2, are typically not restricted from operation well below the critical point. In this lower region, especially when organic modifiers are used, chromatographic behavior remains superior to traditional HPLC and often cannot be distinguished from true supercritical operation.

In analytical SFC, once the separation has been performed and detected, the highly compressed mobile phase is directed through a decompression step to a flow stream. During decompression, the CO2 component of the mobile phase is allowed to expand dramatically and revert to the gas phase. The expansion and subsequent phase change of the CO2 tends to have a dramatic cooling effect on the waste stream components. If care is not taken, solid CO2, known as dry ice, may result and clog the waste stream. To prevent this occurrence, heat is typically added to the flow stream. At the low flow rates of typical analytical systems only a minor amount of heat is required.

While the CO2 component of the SFC mobile phase converts readily to a gaseous state, moderately heated liquid organic modifiers typically remain in a liquid phase. In general, dissolved samples carried through SFC system also remain dissolved in the liquid organic modifier phase.

The principle that simple decompression of the mobile phase in SFC separates the stream into two fractions has great importance with regard to use of the technique in a preparative manner. Removal of the gaseous CO2 phase, which constitutes 50% to 95% of the mobile phase during normal operation, greatly reduces the liquid collection volume for each component and thereby reduces the post-chromatographic processing necessary for recovery of separated components.

A second analytical purification technique similar to SFC is supercritical fluid extraction (SFE). Generally, in this technique, the goal is to separate one or more components of interest from a solid matrix. SFE is a bulk separation technique, which does not necessarily attempt to separate individually the components, extracted form the solid matrix. Typically, a secondary chromatographic step is required to determine individual components. Nevertheless, SFE shares the common goal with prep SFC of collecting and recovering dissolved components of interest from supercritical flow stream. As a result, a collection device suitable for preparative SFC should also be suitable for SFE techniques.

Expanding the technique of analytical SFC to allow preparative SFC requires several adaptations to the instrument. First the system requires increased flow capacity. Flows ranging from 20 ml/min to 200 ml/min are suitable for separation of multi-milligram up to gram quantities of materials. Also, a larger separation column is required. Finally, a collection system must be developed that will allow, at a minimum, collection of a single fraction of the flow stream which contains a substantially purified component of interest. In addition, there frequently exists a compelling economic incentive to allow multiple fraction collections from a single extracted sample. The modified system must also be able to be rapidly reinitialized either manually or automatically to allow subsequent sample injection followed by fraction collection.

Several commercial instances of preparative SFC instrumentation have been attempted which have employed different levels of technology to solve the problems of collection. A representative sampling of these products includes offerings from Gilson, Thar, Novasep, and ProChrome. However, no current implementation succeeds in providing high recovery, high purity, and low carryover from sample to sample. For example, one system may use the unsophisticated method of simply spraying the collection stream directly into a large bottle, which results in high sample loss, presumably due to aerosol formation. Another system uses a cyclonic separator to separate the two streams, but provides no rapid or automated means of washing the separators to prevent carryover. Such instruments are typically employed to separate large quantities of material by repetitive injection so that no sample-to-sample cleaning step is required. Other systems use a collection solvent to trap a sample fraction into a volume of special solvent in a collection container. This technique uses relatively large quantities of hazardous solvents to perform sample collection, is prone to sample fraction concentration losses or degradation, and possible matrix interferences exist between fractionated samples and collection solvent constituents.

An example of a SFC system is illustrated outside of the outlined section

10

in FIG.

1

. The schematic flow diagram is a packed-column supercritical fluid chromatography (SFC) system from initial modifier supply to a detector. The system has a carbon dioxide supply tank

200

, line chiller

220

, pump

202

, modifier tank

204

and pump

206

, dampener and pressure transducer

208

, leading to a mixing column

210

, connected to an injection valve

212

that is connected to at least one packed chromatography column

214

, and a detector

216

.

In a SFC system, liquefied compressed carbon dioxide gas is supplied from cylinders

200

. High pressure tubing

218

connects the carbon dioxide reservoir tank

200

to the carbon dioxide pump

202

. The tubing may be cooled

220

prior to connecting to the pump

202

. The system uses two HPLC-type reciprocating pumps

202

,

206

. One pump

202

delivers carbon dioxide and the other pump

206

delivers modifier

204

, such as methanol. The carbon dioxide and modifier are combined, creating a mixture of modifier dissolved into the supercritical fluid.

The combined supercritical fluid is pumped at a controlled mass-flow rate from the mixing column

210

through transfer tubing to a fixed-loop injector

212

where the sample of interest is injected into the flow system. The sample combines with the compressed modifier fluid inside the injection valve

212

and discharges into at least one packed chromatography column

214

. After fractionation of the sample occurs in the columns

214

, the elution mixture passes from the column outlet into a detector

216

.

SUMMARY OF THE INVENTION

It is an object of the present invention to provide a fraction collection device for supercritical fluid flow systems.

It is a further object of the present invention to provide a device that collects fractionated components of sample solutes into one or more collection containers.

The present invention relates to sample recovery after separation by supercritical fluid chromatography or supercritical fluid extraction, and improvements therein.

More specifically, the present invention relates to optimally separating a liquid phase, containing sample components of interest, from a much larger gaseous phase after the controlled expansion, or decompression, of a single chromatographic mobile phase from a high working pressure to a lower pressure where it is unstable. The controlled decompression causes a phase separation between liquid and gaseous phases while at the same time aerosol formation is strongly suppressed within the transfer tubing.

It is a further object of the present invention to provide a device and method to separate monophasic fluids that are mixtures of highly compressed or liquefied gasses and organic liquid modifiers into gaseous and liquid phases inside transfer tubing prior to collection of fractions of the liquid phase into one or more unique collection chambers. The collection of fractions of the liquid phase into collection chambers minimizes liquid solvent use and waste through efficient gas and liquid phase separation prior to entering collection chambers. The collection technique uses no additional solvents for collection of fractions.

This invention provides a cassette bank of multiple chambers to collect and store separated or extracted fractions. Each collection cassette includes one or more collection chambers, and each chamber can receive a purified liquid fraction. Each chamber may hold a removable sample collection liner. The collection liners may be individually removed, substituted, stored, cleaned and re-used, or discarded. One purpose of the collection liner is to provide a simplified means of transporting the collected liquid fraction from the cassette. A second purpose of the collection liner is to provide a means to eliminate cross-contamination of consecutive samples by providing an easily replaceable, uncontaminated liner in each collection chamber for each sample.

The present invention manually or automatically controls one or more valves and a sealing mechanism for collection chambers such that multiple liquid phase fractions from one sample may be collected into one or more chambers without mechanically adjusting the collection chamber seals. This method allows for rapid switching between collection chambers in the event of closely separated peaks in the chromatograghic flow stream.

It is a further object of the present invention to facilitate a manual or automatic reset of the collection system to allow consecutive samples to be processed in a rapid manner. Technical difficulties arise in the implementation of a collection system that satisfies all the analysts objectives stated above. The major problem centers around the tremendous expansion (typically 500-fold) of the pressurized liquid or supercritical CO2 fraction of the mobile phase that violently transforms into a gas at atmospheric pressure. This transition has four major negative effects with regard to liquid phase sample collection.

First, as mentioned above, the expanding CO2 causes a severe temperature drop that has the possibility of forming dry ice and clogging the system. Since flows of preparative SFC systems are much higher than corresponding analytical systems, considerable more heat must be added to compensate for the temperature drop. Care must be taken; however, not to allow the actual temperature to rise in the flow system since this may cause damage to thermally unstable compounds of interest. Higher organic modifier content reduces the severity of this problem, both by adding heat capacity and by dissolving the CO2, thereby preventing dry ice formation.

Second, as the CO2 expands, it rapidly loses any solvating power it had in the compressed state. If components of interest are largely dependent on the CO2 for solubility they will lose their primary means of transport through the flow system. Solid components will accumulate and eventually clog the flow path causing system failure. Again, the organic modifier component is an important factor here since the liquid will continue to solvate the components of interest and transport them to a collection device. Care must be taken not to introduce too much heat into the flow stream as to drive the organic modified also into the gas phase, otherwise its beneficial effect of transporting the solutes will be lost.

Third, it is beneficial to complete the transition from liquid to gaseous CO2 in as short a period as possible after the initial decompression stage. While in the liquid state, CO2 can disperse the organic modifier containing components of interest even when it is not dense enough to have any significant solvating power. This dispersion can have the effect of remixing components that had been efficiently separated by the SFC process prior to decompression. The faster the CO2 can be converted the less chromatographic degradation can occur. Two factors seem to predominate in controlling the ability to volatilize the liquid phase CO2: a) efficient heat transfer between the heat source and the flowing liquid and b) residence time of the CO2 in the heated region. The first factor can be positively affected by selection of a highly conductive material such as copper for heater fabrication. Insuring excellent thermal contact between the heater and a thin-walled transfer tubing also facilitates heat transfer to the flowing fluids. Residence time of the decompressing fluid can be controlled by stepping the pressure drop over a series of one or more restrictors in the transfer line. Higher backpressure slows the linear velocity of the biphasic fluid in the heater. So long as the back pressure generated by these restrictions do not interfere with the SFC density regulation in the high pressure separation region, a great deal of tunability is possible for optimizing heat transfer.

Fourth, due to the expansion, linear velocities of the depressurizing fluid increase dramatically in the transfer tubing. Residual liquids of the system are moved along the flow path largely by shear forces from the expanding gas. This turbulent environment is ideal for the creation of aerosols, whereby very small droplets of modifier liquid are entrained in the gas phase as a “mist”. It is a finding of this study that the aerosol formation within the transfer tubing can be almost completely controlled by proper temperature control of the expanding two-phase system. Aerosol formation is a greater problem at lower temperatures. It is a surprising finding of this work that higher levels of organic modifier with correspondingly lower CO2 content require higher temperature levels to prevent visible aerosol formation.

In the preferred exemplary embodiment, the SFC collection system is composed of a moderately restrictive, thermally regulated stainless steel transfer tube which extends from a back pressure regulation component of the SFC chromatograph into a multi-port distribution valve and from the valve to a variety of flowpaths leading either through discrete collection chambers or directly connected to a vented common waste container.

Initial separation of the liquid phase sample from carbon dioxide gas occurs immediately at the point of initial decompression within the backpressure regulator of the SFC or SFE instrument. By providing downstream restriction, a minimum backpressure sufficient to prevent the formation of solid CO2 can be maintained while liquid CO2 is present in the transfer lines.

The remainder of the CO2 evaporation and separation from the organic modifier occurs in the stainless steel transfer tubing prior to entering the cassette. This is accomplished by exposing the transfer tubing to a series of one or more heaters designed to optimize thermal transfer to the fluid. Ideally, this heater series transfers sufficient energy to the liquid CO2 portion of the emerging fluid to allow for complete evaporation of the liquid CO2 and raise the fluid temperature sufficiently to prevent the transfer tubing from icing externally. Because rates of heat transfer are time dependent, it is beneficial to slow the velocity of fluids within the heater series.

During the CO2 evaporation process within the first heated zone, significant separation between the gaseous CO2 and liquid modifier occurs. However, the separation to pure CO2 and pure organic modifier is never realized for several reasons. First, some organic modifier is typically also evaporated into the gas state. The degree of evaporation is largely dependent on the absolute temperature of the fluids within the transfer tubing. While organic modifier evaporation does lead to lower recovery of liquid phase, it does not necessarily reduce the recovery of dissolved components of interest which do not typically have low enough boiling points to convert to vapor. Second, a fraction of CO2 will remain dissolved in the organic liquid. Both temperature and pressure determine the amount of residual CO2. Higher temperatures reduce CO2 solubility while higher pressures increase CO2 solubility.

Aerosol formation of the liquid phase is a common problem in SFC sample collection and is a primary cause of loss of the organic liquid phase that contains the dissolved components of interest. Higher temperatures reduce the aerosol generation. The composition of the separated phases also is a factor. Higher temperatures are required to eliminate aerosols in streams with higher organic liquid composition. An additional heated zone is used to trim the fluid temperature to control aerosols. In addition, this heater provides a fine level of temperature control of the fluid before collection in the pressurized collection chamber. As mentioned above, a secondary effect is that a higher trim temperature can reduce the concentration of dissolved CO2, thereby reducing the possibility of uncontrolled or explosive outgassing of the CO2 when the pressure is removed from the collection chamber.

Following the trim heater, a valve system is used to divert the biphasic flow stream sequentially to waste or to one of the collection chambers in a collection cassette. The valve system is comprised of one or more valves and an electronic controller. The system is designed to offer rapid response to a manual or automated start/stop signal. Typically, the signal would result from detection of a component of interest emerging from the high-pressure flow system. A start signal would be generated at the initial detection of the component while a stop signal would be generated at the loss of detection. The effect of a start signal is to divert the flow to the first unused collection chamber of the cassette. The effect of the stop signal is to divert the flow to waste. Another possible type of start/stop signal may be based on a timetable rather than physical detection of components. The controller may also have features to limit the access time or flow volume allowed to an individual chamber. In addition, the controller may allow or prevent the system from cycling back to the original chamber if more fractions are desired than there exists available collection chambers.

The collection cassette is a resealable apparatus that contains one or more hollow collection chambers open at the top. In the preferred exemplary embodiment, each chamber holds a removable inert liner. The liner collects a fraction of the original sample dissolved in a liquid solvent base. A preferred exemplary embodiment of a cassette has four chambers housing four test tube vials that function as chamber liners. The number of chambers in a cassette may be varied with no effect on performance. Each test tube vial may hold up to its capacity of a separated sample fraction from the high-pressure flow stream.

In the preferred embodiment, sample fractions are collected in one chamber of the cassette at a time. The biphasic fluid enters a chamber via a transfer line from the valve system. The tip of the transfer line is preferentially positioned tangential to the inner wall of the collection tube and with a slight downward angle, usually less than 45 degrees from horizontal. Attached to the transfer line and suspended inside a test tube is a guiding spring wire. The spring wire is bowed away from the transfer line and functions as a guide for the transfer line as it descends into a vial. When transfer tubing is properly inserted into a test tube vial, the bowed section of the spring wire engages the circumferential edge of the open end of a test tube vial. As the tubing continues into the test tube, the spring wire compresses against the inner surface of the test tube vial and pushes the tubing towards the opposite side of the vial. As a result, the angled tip of the transfer tubing is pressed against the inner wall of the test tube vial.

Both the organic liquid and CO2 gas follow a descending spiral path along the inner wall to the bottom of the collection liner. The liquid collects at this point and begins to fill the liner. The CO2 gas continues in a path up the center of the liner to a vent in the collection chamber. A restrictive transfer line attached to the vent causes the CO2 gas to pressurize the collection chamber both inside and outside the collection liner. The degree of back pressurization within the chamber is roughly proportional to the composition of CO2 in the original mobile phase.

The pressurization of the collection chamber serves to slow down the velocity of the CO2 entering the chamber. This in turn reduces the magnitude of shear forces occurring between the CO2 gas and the collected liquid at the bottom of the liner. With lower shear forces, there is less tendency for the collected liquid to become an aerosol and to be removed from the collection tube with the exiting gas. A similar effect is obtained by the proper angling the inlet transfer line relative to the collection tube wall. The closer the angle of the tube is to horizontal the lower the observed turbulence at the liquid surface. However, enough angle must be provided to insure the majority of effluent is directed downward rather than upward on the liner wall. The two effects of back pressure and delivery angle combine to reduce aerosol formation in the collected liquid fraction. The success of optimizing these effects determines how close the inlet tube can come to the collection liquid, and thereby determining how high the liner may be filled before sample loss becomes a problem. When flow to the chamber is stopped, the chamber depressurizes. Once the sample chamber is depressurized, the liner may be removed by opening the top lid of the cassette.

The collection of fractions into disposable liners of collection chambers may be automated through the use of robotics. An automated system enables rapid substitution of test tube vials into and out of collection chambers and long unattended run times based on a quantity of vials available for substitution. A programmable robot automatically sequences cassettes between sample injections, thereby speeding up the process while reducing the margin for error. The automated system can collect on the order of thousands of fractions per month.

The automated system is contained in laboratory grade housing. The system is comprised of a robotic arm, a supply of test tube vials arranged upright in racks, and an automated version of a cassette assembly. In addition, the system may contain sufficient probes, valves and sample containers to achieve automated delivery of unfractionated samples into the chromatographic or extraction system.

The collection cassette and its automated mechanisms are designed for rapid sample collection and minimal stop time between chamber liner replacements. The cassette in the preferred embodiment has two banks of four collection chambers each. A lid is positioned above one bank of collection chambers in the cassette. The lid has four partially recessed annular bores corresponding to the four collection chambers in the cassette. The lid raises and lowers with action from pneumatic actuators mounted on the base of the housing and located on opposite longitudinal ends of the lid. As the actuators simultaneously lower the lid onto the collection cassette, the top edge of each chamber engages the bottom edges of the lid corresponding to the rims of each partially recessed bore. The lid and chambers engage and form pressure tight seals in each chamber in preparation for sample fraction collection. The lid has transfer and waste line tubing passing through each recessed bore that correspond to each collection chamber. Each tubing pair enters a test tube as the lid is lowered onto the cassette. The spring wire attached to the inlet tubing guides an inlet tube into a test tube vial. An angled tip on the tube is forced against the inner wall of the test tube. After the lid has sealed on the row of collection chambers, a valve system dispenses the flowstream containing gaseous and liquid phases into the chamber liners from the sample fractionation process.

When all test tube vials in the pressurized cassette row have been filled and depressurized, the lid lifts off of the cassette. The cassette then moves laterally, or shuttles, until a row containing empty collection chamber liners is moved under the lid in place of the former row. The cassette is constrained to shuttle laterally along a path on the base of the housing. The lid lowers and engages the new row of chambers, thereby preparing the test tubes to accept sample fractions. Meanwhile, the former row of chamber liner test tube vials containing liquid fractions are removed from the collection chambers and transported to open spaces in a storage tray via a robot arm.

In summary, samples in the preferred embodiment are dissolved in a minimum volume of modifier solvent and are collected in removable and reusable liners. Through controlling flowrate, velocity, temperature, and pressure in the system, superior separation of near-supercritical elution fluid is obtained. Collection efficiencies of up to 98% of injected sample components may be realized. The cassette, by utilizing pressurized collection chambers and disposable liners in the process, minimizes the use of additional collection and cleaning solvent spent by a laboratory, which is economical and good for the environment. Laboratories and research facilities that demand purity of samples while maximizing output and minimizing waste will benefit from the proposed invention. Large-scale sample fractionation and collection, numbering in the thousands of samples per month, may be realized from the exemplary embodiment.

BRIEF DESCRIPTION OF THE DRAWINGS

For a better understanding of the nature of the present invention, reference is had to the following figures and detailed description, wherein like elements are accorded like reference numerals, and wherein:

FIG. 1

illustrates a schematic flow diagram of the supercritical fluid chromatography system and the collection system including the sample cassette embodied in the invention.

FIG. 2

illustrates an exploded isometric view of a sample collection cassette.

FIGS. 3A and 3B

illustrate top and bottom plan views of the cassette lid.

FIG. 4

illustrates a plan view of an alternative exemplary embodiment of an automated fraction collection system.

FIG. 5

illustrates a side view of an alternative exemplary embodiment of an automated fraction collection system.

FIG. 6

illustrates an exploded isometric view of a shuttle sample collection cassette, lid, and mechanized controlled movement system.

FIG. 7

illustrates a detailed side view of the shuttle cassette and associated mechanical control apparatus.

FIGS. 8A and 8B

illustrate detailed cross sectional views of transfer tubing before and after insertion into a test tube vial.

FIG. 9

illustrates an alternative embodiment of an integrated collection cassette having multiple rows of collection chambers.

FIG. 10

illustrates an additional alternative embodiment of a shuttle collection cassette for an automated system.

DETAILED DESCRIPTION OF PREFERRED EXEMPLARY EMBODIMENTS

The preferred embodiment of the apparatus is illustrated in the flow chart of

FIG. 1

within the perimeter line

10

. Except where noted, specifications for a preferred exemplary embodiment are given for a system that accepts flows of 20 to 100 mL/min total flow (CO2 plus modifier flow) in the highly compressed state from the pumping system. Flowrates for alternative embodiments could range in orders of magnitude higher or lower through adjustment or substitution of system hardware and flow parameters.

In the preferred exemplary embodiment, the SFC collection system is composed of a moderately restrictive, thermally regulated transfer tube

12

which extends from a back pressure regulator

14

into a multi-port distribution valve

22

and from the valve to a variety of flowpaths leading either through discrete collection chambers

32

or directly connected to a vented common waste container

26

.

Expanded elution fluid leaves the backpressure regulator

14

at a velocity of approximately two to five times the flow velocity upstream of the backpressure regulator

14

and under back pressure of approximately twenty to forty bars. Variations in the expansion occur as a result of the changing modifier solvent concentration from 2.5 to 50 percent over the course of a separation.

Initial separation of the liquid phase sample from carbon dioxide gas occurs immediately at the point of initial decompression within the backpressure regulator

14

of the SFC or SFE system. By providing downstream restriction, a minimum backpressure sufficient to prevent the formation of solid CO2 can be maintained while liquid CO2 is present in the transfer lines

12

. The degree of CO2 evaporation is a function of both the available heat transfer in this region and the downstream flow restriction which limits the amount of expansion available to the decompressing fluid. Due to the pressure drop across the backpressure regulator

14

, a fraction of the emerging CO2 will evaporate, typically causing a significant drop in the temperature of the emerging fluid.

Further separation and evaporation of CO2 from the organic modifier occurs in stainless steel transfer tubing

12

running between the first backpressure regulator

14

and the cassette

24

. The transfer tubing

12

containing a flowstream of the biphasic CO2 and modifier is exposed to a series of a heaters

16

,

18

designed to optimize thermal transfer to the biphasic fluid in the flowstream. Ideally, this heater series transfers sufficient energy to the liquid CO2 portion of the emerging fluid to allow for complete evaporation of the liquid CO2 and raises the fluid temperature sufficiently to prevent ice from forming externally on the transfer tubing

12

.

During the CO2 evaporation process within the first heated zone, significant separation between the gaseous CO2 and liquid modifier occurs. However, the separation to pure CO2 and pure organic modifier is never realized. Some organic modifier is typically evaporated into the gas state. The degree of evaporation is largely dependent on the absolute temperature of the fluids within the transfer tubing

12

. While organic modifier evaporation does lead to lower recovery of liquid phase when it reaches the collection cassette

24

, it does not necessarily reduce the recovery of dissolved components of interest which do not typically have low enough boiling points to convert to vapor. A fraction of CO2 will also remain dissolved in the organic liquid modifier. Both temperature and pressure determine the amount of residual CO2. Higher temperatures reduce CO2 solubility while higher pressures increase CO2 solubility. Turbulent flow of the CO2 gas within the narrow tubing also produces a strong shearing force that propels the liquid down the walls of the transfer tube

12

. This very turbulent flow frequently causes small droplets at the liquid surface to rip away from the bulk liquid and become entrained into the rapidly moving gas phase of the fluid down the transfer tube

12

. Such an effect is called aerosol formation, or “misting”.

A plurality of heaters may be mounted in series to heat the elution fluid. In

FIG. 1

, the preferred exemplary embodiment has an evaporator heater

18

and a trim heater

20

mounted in series after the backpressure regulator

14

. The evaporator

18

is heated with an appropriately sized cartridge heater and controlled by an appropriate heater controller. In the preferred embodiment, transfer tubing

12

is tightly coiled around the heating assembly and optimized for thermal contact. The elution fluid is heated to within the control temperature of the evaporator

18

, which is between approximately 5 to 50 degrees C., to protect heat sensitive compounds from being damaged. The objective is to boil CO2 out of the elution fluid as the fluid passes through the evaporator

18

. To complete the required heat transfer, biphasic elution fluid inside transfer tubing

12

enters the final heat exchanger, which is a trim heater

20

. In the preferred embodiment, the trim heater setting is typically above the evaporator

18

setpoint. The heater

20

is used not only to suppress aerosol formation within the transfer tube

12

but also to control the level of dissolved CO2 in the liquid phase.

It is beneficial to slow the velocity of fluids within the transfer tubing

12

passing through the heater series

18

,

20

. The fluid velocity is slowed inside the transfer tubing

12

by placing a restrictive orifice or smaller diameter tube immediately downstream from first heater series. Elution fluid exits the evaporator

18

and enters a flow restrictor

16

, which provides a higher backpressure in the evaporator

18

and thereby slows the flow and increases the contact time of the liquid CO2 phase. The restrictor

16

also insures a high enough backpressure to prevent the liquid carbon dioxide from forming solid carbon dioxide, also known as dry ice. The restriction increases the backpressure in the heated zone and reduces the amount of the gas expansion. In an alternative exemplary embodiment, the velocity of fluids can be slowed after all heaters, however such a configuration does not control the final expansion of CO2 which can result in uncontrolled cooling of fluids within the transfer lines. As a result, the ability to actively suppress aerosol formation may be diminished.

After exiting the trim heater

20

, transfer tubing

12

connects to the common port of a valve system

22

. The valve system in the preferred exemplary embodiment is a multi-port selector valve

22

. As elution fluid from the peak of interest passes through the valve system

22

, the gas and liquid phases are directed into either a collection cassette

24

or to a waste stream container

26

. The outlet ports on a multi-port selection valve

22

are connected to a plurality of transfer tubing lines

28

. The transfer lines

28

pass through a cassette lid

30

and into discreet chambers

32

within the cassette

24

. The transfer lines

28

have airtight and pressure resistant connections into and out of the cassette lid

30

. The remaining ports in a multi-port selection valve

22

connect to waste transfer lines

34

. In an alternative exemplary embodiment, multiple discreet valves are installed and connected to the incoming transfer line

12

, having each valve port connected to an individual collection chamber

32

in the cassette

24

and a discreet valve connected to a waste line

34

.

Inlet lines

28

entering a collection chamber

32

insert into a test tube vial

36

within a chamber

32

. Liquid phase

38

is captured in a test tube

36

while gaseous phase escapes out of a chamber

32

through a discharge line

40

. Gas in the discharge line

40

is flowing at high pressure. Discharge lines

40

from the cassette

24

run through a pressure relief switch

42

to protect the cassette and upstream components from possible damage due to over-pressurization from a system malfunction.

Referring additionally to

FIG. 2

, a preferred exemplary embodiment of the cassette

24

comprises four discreet collection chambers

32

. However, in alternative embodiments, one or more individual chambers

32

are possible in the cassette

24

. Each collection chamber

32

in the preferred embodiment is a closed system that is the final separation point of liquid and gaseous phases. Chambers

32

are hollow cylinders constructed of high strength transparent plastic to allow visual monitoring of separation and collection processes. The cassette chambers

32

can be formed of stainless steel or other appropriate laboratory-grade materials. The chambers

32

sit parallel and upright in the cassette

24

. Each chamber

32

is constrained at its upper and lower ends within a molded frame

44

,

46

. Each chamber

32

is set with the open end surrounded by the upper molded frame

44

and the lower end partially embedded into the lower molded frame

46

. Communication of liquid or gaseous phases between chambers

32

is prohibited by seals

48

that are seated in a groove

50

at the top, open end of each chamber

32

.

Each collection chamber

32

houses a removable, replaceable liner. A standard glass test tube vial

36

functions as a liner and is seated upright inside each the chamber

32

. The closed bottom of a test tube vial

36

rests on the base of the chamber

32

and is easily removable. Once inserted, the top of the test tube vial

36

must be lower than the combined height of a chamber

32

and the internal recessed bore

60

(

FIG. 3

) of a lid piece

30

when the lid and cassette

24

are engaged. A test tube vial

36

and a chamber

32

are a single pressurized system that communicate through the top of the chamber

32

. The test tube vial

36

functions as a disposable liner for the chamber

32

to capture the liquid phase

38

that has separated from the flow stream. The inside of the vial

36

and the annular space of the chamber

32

surrounding the vial are equilibrated to the same pressure, which is a range of approximately 20 to 100 psig during separation processes for a flowstream up to 50 ml/min. This arrangement enables sample fraction collection at high pressure using standard laboratory glass test tube vials

36

without a risk of breaking the glass vial inside the chamber

32

.

FIG. 2

illustrates the cassette

24

, comprising a rectangular frame securing four upright chambers

32

. The upper section

44

and lower section

46

of the molded frame hold the chambers

32

in place. The frame is completed by two rigid rectangular end pieces

52

attached to the upper and lower sections. Each end piece

52

is a metal plate fastened to the upper

44

and lower

46

frame sections with machine screws

54

. Butterfly latches

56

are installed at the top of both rigid end pieces

52

secure the lid piece

30

to the top of the cassette

26

. The lid

30

may be removed manually between sample injections for quick access to, and removal of, chamber liners

36

. As illustrated in

FIG. 1

, the bottom of each chamber

32

has a transfer tube or orifice

33

running completely through the base of a collection chamber and lower frame

46

. The orifice

33

through the chamber base

46

can be used to remove liquid phase fluid from a chamber

32

without opening the chamber or depressurizing the chamber

32

. The sample discharge port

33

also permits easier draining and cleaning of the chamber

32

during maintenance of the cassette

24

.

FIGS. 3A and 3B

illustrate top and bottom views of the removable cassette lid

30

, respectively. The lid

30

has four sets of three boreholes

58

in a triangulated pattern positioned such that each set of boreholes is directly over each of the chambers

32

when the lid

30

is engaged to the cassette

24

. The bottom face of the lid

30

has partially recessed bores

60

positioned directly above each chamber

32

when the lid

30

and cassette

24

are engaged. The diameter of a recessed bore

60

is sized slightly smaller than chamber

32

diameters. The recessed bore's

60

perimeter is positioned completely inside of a seal

48

when the lid

30

is fastened to the cassette, as illustrated in FIG.

2

. The recessed boreholes

60

allow a test tube

36

to stand taller than the top planar surface of the upper frame section

44

of the cassette

24

so that a test tube

36

may be removed without reaching into a collection chamber

32

, thereby possibly cross-contaminating subsequent samples. To guide the lid

30

and cassette base

24

together when engaging, alignment pins

62

, illustrated in

FIG. 3

, are formed on the outer, top surface of the cassette frame

24

. Partially recessed bores

63

in the lid

30

receive the alignment pins

62

from the cassette frame

24

. Catches

64

for the butterfly latches

56

are attached to each long end of the lid

30

.

Inlet transfer tubing

28

carries liquid and gaseous phases into test tube vials

36

housed in each collection chamber

32

of the cassette. Each inlet tube

28

fits through a hole

58

in the lid

30

and inserts into a test tube vial

36

. Proper fittings on the tubing

28

provide airtight connections that can also withstand pressure forces in the SFC system. Inlet tubing probes

66

direct elution fluid into a test tube vial

36

and an outlet tube

68

provides an escape route for gas that is under pressure to exit the chamber

32

and discharge to waste collection

26

.

In the preferred embodiment, fractions are collected in one chamber

32

of the cassette

24

at a time. During the fractionation process, both the liquid phase and the gas phase discharge into the collection vial

36

where final separation takes place. The pressurization of the collection chamber

32

serves to slow down the velocity the CO2 within the chamber

32

. This in turn reduces the magnitude of shear forces occurring between the CO2 gas and the collected liquid at the bottom of the liner

36

. With lower shear forces, there is less tendency for the collected liquid to become an aerosol and removed from the collection liner

36

with the exiting gas. A similar effect is obtained by the proper angling the inlet transfer line relative to the collection liner

36

wall. The closer the angle of the tube

66

is to horizontal the lower the observed turbulence at the liquid surface. However, enough angle must be provided to insure the majority of effluent is directed downward rather than upward on the liner

36

wall.

The biphasic elution fluid enters a chamber

32

via a transfer line

28

from the valve system

22

. As illustrated in

FIGS. 8A and 8B

, the tip of the transfer tube

66

is a probe preferentially positioned tangential to the inner wall of the collection vial

36

and with a slight downward angle, usually less than 45 degrees from horizontal. Attached to the probe

66

is a guiding spring wire

70

. The spring wire

70

is bowed away from the probe

66

. The spring wire

70

acts as a guide for the probe

66

as the probe descends into a test tube vial

36

. When the probe

66

is properly inserted into a test tube vial

36

, the bowed section of the spring wire

70

contacts the circumferential edge of the open end of a test tube vial

36

. As the tubing

66

continues into the test tube vial

36

, the spring wire

70

compresses against the inner surface of the vial

36

and pushes the probe

66

towards the opposite side of the vial

36

. As a result, the angled tip of the probe

66

is pressed against the inner wall of the test tube vial

36

.

The spring wire

70

is extruded from inert materials that will not chemically interfere with collected samples in the test tube vials

36

. In an alternative exemplary embodiment, the probe section

66

of the transfer tubing

28

is a rigidly held stainless steel probe attached to the cassette lid

30

. Metal versions of probe

66

may be terminated with a larger OD Teflon tube sleeved onto the metal probe to prevent scratching and possible rupture of the inner wall of the collection liner

36

.

Both the organic liquid and CO2 gas follow a descending spiral path along the inner wall to the bottom of the collection liner

36

. The liquid phase collects at this point and begins to fill the test tube vial

36

. The CO2 gas continues in a path up the center of the vial

36

to a vent through the top of the collection chamber

32

. A restrictive transfer line attached

72

to the vent causes the CO2 gas to pressurize the collection chamber

32

both inside and surrounding the collection liner

36

. The degree of back pressurization within the chamber is roughly proportional to the composition of CO2 in the original mobile phase.

The two effects of back pressure and delivery angle combine to reduce aerosol formation in the collected liquid fraction. The success of optimizing these effects determines how close the inlet tube

66

can come to the collection liquid, and thereby determining how high the liners

36

may fill before sample loss becomes a problem. When flow to the chamber

32

is stopped, the chamber depressurizes. Once a chamber

32

is de-pressurized, the test tube vial

36

containing liquid phase may be removed by opening the top lid

30

of the cassette

24

.

The outlet line tubing

72

from each chamber

32

is connected to a fixed restrictor

42

to keep pressure inside the chambers

32

. The fixed restrictor

42

raises the upstream pressure between approximately 20 and 100 psig depending on CO2 flow rate. Each discharge line

72

passes through a pressure switch

78

to protect against overpressuring and rupturing. Pressure in each chamber is monitored visually with a pressure gauge

76

that is threaded into the lid

58

over each chamber

32

. Discharge lines

72

are directed to a waste collection tank

26

, from which the CO2 is vented. To increase laboratory safety, the system should not have any exposure of waste effluent, samples, or vented CO2 to ambient laboratory air. The liquids and gasses in the system remain in a contained system that can be directed to a hood or safety exhaust

26

to maximize safety for the technician.

The volume of the captured fractionated liquid phase

38

in the collection vial

36

is controlled manually or automatically. Automatic control in the preferred exemplary embodiment of the valve system

22

and is comprised of one or more valves and an electronic controller. The valve system

22

is designed to offer rapid response to a manual or automated start/stop signal. A signal can result from detection of a detection of a component of interest emerging from the high pressure flow system. A start signal would be generated at the initial detection of the component while a stop signal would be generated at the loss of detection. The effect of the stop signal is to divert the flow to waste lines

26

or to another chamber

32

. An alternative embodiment of a type of start/stop signal may be based on a timetable rather than physical detection of components. The controller may also have features to limit the access time or flow volume allowed to an individual chamber

32

. In addition, the controller may allow or prevent the system from cycling back to the original chamber

32

if more fractions are desired than there exist available collection chambers

32

.

An alternative exemplary embodiment of the collection cassette and system is illustrated in

FIGS. 4 through 7

. This embodiment is an automated system that utilizes a robotic arm

80

to replace chamber collection liners

36

after filling with sample fractions. The robotically controlled unit is designed for rapid filling and replacement of chamber liners

36

combined with a long unattended run time. Supply trays

86

of clean test tube vials

36

that function as chamber liners

36

are located within the unit's housing

82

. A robotic arm

80

is controlled to replace one or more liners

36

from a row of collection chambers

32

in a collection cassette

84

with liners

36

from a fresh supply rack

86

. The robotic arm

80

is mechanized to replace liners

36

on a first row of the cassette

84

while liners

36

on a second row are automatically moved into place. This robotically automated alternative embodiment provides faster sample collection through a minimum of down time to replace liners

36

as well as the ability to collect a greater number of samples during an unattended session.

FIGS. 4 and 5

illustrate the plan and side views, respectively, of an automated alternative exemplary embodiment of the SFC sample collection system. The components for the system are partially enclosed with a laboratory-grade housing structure

82

having a raised mounting base

88

within the housing

82

. The housing

82

is supported with adjustable feet

90

that are distributed around the base of the housing

82

. The feet

90

adjust the level the housing

82

to compensate for uneven or slanted surfaces. Supplies of uncontaminated test tube vials

36

are stored in racks

86

placed on a raised interior base

88

of the housing

82

. Each test tube vial

36

is held upright and secured in-place in a rack

86

by molded supports. Each support rack

86

consists of circular sections attached tangentially to neighboring sections, forming multiple rows and columns. The molded supports loosely secure test tube vials

36

that are held in each circular opening of the racks

86

. The vials

36

are maintained equidistant from each neighboring vial to provide adequate spacing for a grabbing jaw

92

on a robotic arm

80

to grasp a vial

36

without interference from a neighboring vial. The spacing also prevents chipping or breakage during movement and replacement of the rack

86

. Two racks

86

of test tube vials

36

are illustrated in the Figures, however the system could easily expand to a plurality of racks of the vials

36

.

An alternative exemplary embodiment of a cassette

84

and associated system devices is installed on the raised interior base

88

. The cassette

84

has a plurality of rows of chambers that are constrained to lateral movements that are automatically controlled with a pneumatic actuator

96

. This cassette

84

is termed the “shuttle cassette”, or simply “the shuttle.”

FIGS. 6 and 7

illustrate the shuttle cassette

84

in isometric and side views, respectively. The shuttle cassette

84

is constructed similar to the exemplary embodiment with an added row of collection chambers

102

. The shuttle

84

comprises upper and lower rectangular molded frames

98

,

100

supporting a plurality of rows of upright cylindrical collection chambers

102

. The shuttle

84

is constructed with two rows of four cylindrical collection chambers

102

in each row. The size of the shuttle

82

can be modified to add additional rows of chambers

102

or additional chambers per row, such as an alternative embodiment featuring three rows of chambers

102

illustrated in FIG.

10

. The shuttle cassette

84

is formed on two opposite ends with rigid rectangular plates

104

. Each end plate

104

is fastened to the upper

98

and lower

100

molded frame sections with machine screws

106

. The shuttle

84

may be constructed with permanent attachments and fittings, however, a shuttle that readily disassembles allows easier and thorough cleaning and replacement of worn or damaged components.

The collection chambers

102

are formed of high-strength transparent plastic, which allows visual monitoring of the collection process inside of each chamber

102

. As an alternative, the chambers

102

may be formed of stainless steel or a similar high-strength material compatible with SFC parameters described herein. Each cylindrical chamber

102

is set into the lower molded frame

100

for base support. The upper molded frame section

98

is secured near the open, top end of each chamber

102

. Each chamber

102

extends above the top surface of the shuttle

84

at a standardized distance adequate to seal the chambers

102

with an automated lid piece

108

. Standard laboratory test tube vials

36

may be inserted into each of the chambers

102

to act as a removable or disposable liner for each chamber.

The automated shuttle cassette

84

is constrained to lateral movements on the inner raised base

88

. The lower molded frame section

100

, or base, of the shuttle cassette

84

has an horizontally bored hole

110

, illustrated in

FIG. 7

, running perpendicular to the open sides of the shuttle. Offset from the shuttle

84

is an actuator

96

installed on the raised base

88

of the housing unit

82

. Attached to the actuator

96

is rod

94

or controller arm. The rod

94

is constructed of a rigid material, such as stainless steel, and inserts into the bored hole

110

in the base of the shuttle cassette

84

, wherein it is firmly attached to the base frame

100

. The actuator

96

executes lateral movements of the shuttle

84

according to commands sent from a programmable control system. In an alternative embodiment, the base of the shuttle

100

has small rollers

112

installed around the base, as illustrated on FIG.

7

. The rollers

112

are guided laterally by grooved tracks in the base of the housing

88

. The tracks not only constrain the movement of the shuttle

84

but also remove tension from the controller arm

94

and actuator

96

gears caused by the shuttle

84

drifting into angled movements caused by uneven friction on the rollers, initial off-center displacement after shuttle

84

installation, or irregularities on the surface of the housing base

88

. Other methods of providing constrained lateral movement are possible in alternative embodiments, such as utilizing guide tracks wherein guides on the shuttle

84

are enclosed within tracks riding on ball-bearings.

Referring to

FIGS. 6 and 7

, the lid

108

of the shuttle cassette

84

is automatically controlled to engage a row of collection chambers

102

after the shuttle is moved into place directly below the lid

108

by the lateral actuator

96

. In the alternative embodiment, the lid

108

is constructed of stainless steel. However, high density plastic, or a similar material having equivalent rigidity and composition for use in the collection system, is sufficient. The lid

108

has a hole

114

through each longitudinal end, bored parallel to the vertical axis of the lid. The holes

114

in each end of the lid

108

are sized to fit a threaded rod

116

. Two nuts

118

threaded above and below the lid

108

secure the lid to each rod

116

. The lid

108

is constrained to move only in the vertical plane. The movements of each rod

116

are controlled by actuators

120

mounted to the raised base of the housing

88

. The two pneumatic actuators

120

controlling the lid movements are synchronized to move the rods

116

vertically, thereby raising and lowering the lid

108

onto a row of collection chambers

102

in the shuttle cassette

84

.

FIG. 7

illustrates the lid piece

108

raised above the shuttle

84

prior to engagement. The bottom face of the lid

108

has four bores

122

partially recessed into the lid corresponding to four chambers

102

in a row of the shuttle. As the lid

108

is lowered by the pneumatic actuators onto the shuttle

84

, each chamber

102

of a row partially inserts into a recessed borehole

122

. The lid

108

stops at a programmed point at which the circular edge of each bore

122

engages and seals against the flat upper surface of the shuttle frame

98

. Each partially recessed borehole

122

in the lid

108

has a diameter larger than the chamber's

102

diameter. As the lid

108

lowers onto the shuttle

84

, the recessed boreholes

122

are lined up with the top, open ends of the chambers

102

. The larger diameter recessed boreholes

122

each totally enclose the open end of each chamber

102

. An appropriate sealing O-ring or similar component is placed around the top of each chamber

102

, between the top of the shuttle

84

and the lid

108

, to provide an airtight and pressure resistant seal when the two components engage. Alignment pins

124

are located on the top surface

98

of a shuttle

84

at both ends of each row of chambers

102

. The pins

124

are shaped as half-spheres on the top surface of the shuttle

84

and provide additional protection for shuttle collection chambers

102

from misalignment of the shuttle

84

to the lid

108

. As the lid

108

engages onto the shuttle

84

, the alignment pins engage corresponding bores

126

in the lid.

A collection chamber

102

is a discreet system that is the final separation point of liquid and gaseous phases. Communication of liquid or gaseous phases between chambers

102

is prohibited through the lid

108

that seals each chamber airtight as it automatically lowers onto a row of chambers in the shuttle cassette

84

. Similar to the exemplary embodiment of the cassette, each chamber

102

in the shuttle

84

holds a chamber liner

36

to catch fractionated liquid phase. The liner

36

is a standard laboratory test tube vial

36

. The closed bottom of the test tube

36

rests at the base of each chamber

102

, which rests on the lower molded frame of a shuttle

100

. A test tube vial

36

and chamber

102

communicate as a single pressurized system.

FIG. 8B

illustrates the position of the open end of a vertically disposed test tube vial

36

below the top of a recessed borehole

122

after the lid

108

engages the shuttle

84

. The inner pressure of the test tube vial

36

and the chamber's

102

annular space surrounding the vial are equilibrated and range from approximately 20 to 100 psig during collection processes. This arrangement enables sample fraction collection at high pressure using standard lower pressure glass or plastic vials by equilibrating the pressure forces inside and outside the vial

36

.

As illustrated in

FIG. 7

, the lower, closed end of each chamber

102

has a sample discharge port

128

running completely through the lower shuttle frame

100

. A plug is inserted into each sample discharge port

128

during regular use of the shuttle

84

. The sample discharge port

128

permits removal of liquid phase that is collected directly into a chamber

102

without using a liner. By withdrawing liquid phase through the sample discharge port

128

, the liquid phase may be collected without disengaging the lid

104

from the shuttle

84

. Liquid phase may be evacuated from a chamber

102

under pressure or gravity fed out of a chamber after chamber depressurization.

Inlet

66

and outlet

68

tubing for transferring influent and effluent liquid and gas phases between the shuttle cassette

84

and external transfer lines are illustrated in

FIGS. 6 and 7

. Inlet

66

and outlet

68

tubing for the shuttle

84

pass through the lid

108

. Transfer tubing

66

,

68

is constructed from high-pressure stainless steel or equivalent materials. Inlet tubes

66

carry gaseous and liquid phases into a collection chamber

102

under high pressure. Outlet tubes

68

carry separated gaseous phase to a waste tank

26

for venting or disposal. The lid section

108

has four sets of three holes

134

in triangular formations that pass through the lid and are located to correspond with collection chambers

102

when the lid is engaged to the shuttle cassette

84

.

In addition to transfer tubing, one of the holes

134

permits measurement of pressure forces inside a chamber with a pressure gauge

76

threaded into the hole

134

from top of the lid

108

. The transfer tubing

66

,

68

and pressure gauge

136

all have pressure resistant airtight fittings specified to withstand pressure forces created in the SFC system. Transfer tubes

66

,

68

installed below the lid

108

insert into a test tube vial

36

when the lid

108

is engaged to the shuttle cassette

84

. The tip of each inlet tube

66

, or probe, is constrained to an angle less than 45 degrees and wrapped with non-reactive spring wire

70

that is bowed along the vertical section, similar in construction and purpose as described in the preferred embodiment. The spring wire

70

serves to angle the inlet tubing

66

inside a test tube vial

36

by applying pressure forces against the vial's

36

inner wall. As a result, the open tip of the inlet tube

66

is forced tangentially against an opposing inner wall of the vial

36

. This configuration of the inlet tube

66

is desirable because it causes the liquid phase that exits the inlet tube

66

to contact a side wall of the vial

36

and swirl down the inner wall of the vial

36

in a spiraling motion. The swirling action provides the final separation process of liquid phase from entrained gaseous phase while preventing re-entrainment and loss of sample fractions from the liquid phases into gaseous phases or aerosol mists that can be carried away with gaseous phases to a waste vent

26

.

In an alternative exemplary embodiment, a robotic arm, such as a Cartesian or three-dimensional robotic arm, is programmably controlled to move test tube vials between supply racks and the shuttle cassette collection chambers.

FIGS. 4 and 5

illustrate a three-dimensional robotic arm

80

mounted to a wall of the unit housing

82

near the shuttle cassette

84

. A host PC or microcontroller issues positioning commands for the arm's movement and controls automated functions. The arm

80

has a jaw

92

to grab and place test tube vials

36

into the shuttle cassette

84

from the test tube supply racks

86

. The jaw

92

is controlled to grip test tube vials

36

of specific outer diameter and at specific locations within the unit

82

. In the alternative embodiment illustrated in

FIG. 5

, the robotic arm

80

is gripping one test tube

36

in its jaw

92

to move the test tube between the shuttle

84

and a supply rack

86

. To increase the volume of vials

36

exchanged, the gripper jaw

92

could be modified to grip two or more test tube vials, multiple jaws could be placed on a single arm

80

, or multiple robotic arms could work on the same embodiment. The arm

80

acts in concert with the automated movements of the shuttle

84

. As a row of chambers

102

in the shuttle

84

is engaged to the lid

108

, the robotic arm

80

replaces test tube vials

36

in the shuttle that are filled with collected sample fractions with fresh vials

36

from a supply rack

86

. When a row of test tubes

36

in the shuttle

84

have been replaced, and the row of vials

36

under the lid

108

have captured liquid phase fractions, a programmable controller signals the pneumatic actuators controlling the lid

120

to disengage and move the lid

108

away from the shuttle

84

. The lateral control

96

of the shuttle

84

is then signaled to move the shuttle such that the row of chambers

102

containing clean, uncontaminated test tube vials

36

correspond to a position underneath the lid

108

prior to engagement. The lid actuators

120

are then signaled to engage the lid

108

again to the shuttle

84

, thereby preparing the chambers to receive liquid phase fractions. The robotic arm

80

next grabs vials

36

from the exposed shuttle chambers

102

that contain liquid phase fractions and places them into a supply rack

86

. The arm

80

then replaces an uncontaminated vial

36

into each empty chamber

102

until a row of chambers is completely filled with fresh test tubes. This process is repeated for the length of a sample run or until the system is depleted of uncontaminated test tube vials from the supply racks

86

.

An alternative embodiment of a collection cassette is illustrated in FIG.

9

. An integrated cassette

140

consists of multiple rows of wells

144

in a grid pattern formed similar to a titration tray. The smaller footprint of the integrated cassette

140

can increase the density of collection chambers over the shuttle cassette

84

. The integrated cassette

140

also functions as a storage tray for gathered liquid phase fractions. Therefore, time and expense are saved during sampling procedures by removing the steps of the substituting chamber liners

36

and replacing liners from a separate storage area. By modifying the lid

108

and mechanics of the automated collection system, the integrated cassette

140

may serve as its own sample collection cassette and storage tray and can rapidly receive fractions without having to replace liners

36

between each sample injection. The robotic arm

80

in the system may replace integrated cassette

140

units as a whole after a sampling event is completed or chamber wells

144

contain the desired amount of liquid phase fractions. A plurality of integrated cassettes

140

are stored in the automated collection system providing the means for hundreds of collected fractions during an automated run. A preferred construction of an integrated cassette is a 4×6 chamber array in the deep-well micro titer plate format used commonly in the pharmaceutical industry. Such a format improves automation storage density not only due to more chambers per area, but these chambers are also easily stackable, which gives an added dimension of sample storage capacity. This alternative embodiment is a shuttle cassette tray

140

formed from high-strength materials such as plastic, resin, or stainless steel.

The integrated cassette tray

140

is also advantageous for rapid fraction collection because it can be modified to contain replaceable liners

36

in the wells

144

or use no liners, thereby collection liquid fractions directly into the wells

144

. The integrated cassette

140

can be replaced as a unit after wells

144

are filled with liquid phase fractions.

An alternative embodiment of an automated system using a cassette tray would appear similar to that illustrated in

FIG. 4

but with certain modifications. Modifications to the automated system include spacing for a supply of cassette trays

40

instead of test tube racks

86

, sizing of the lid piece

108

and associated mechanized controllers

120

and transfer tubing

66

,

68

, sizing of lateral mechanized controllers

96

for the tray

140

while switching between rows of chambers

144

during fraction collections, and modification of a robotic arm

80

to substitute filled cassette trays

140

with new trays from a supply area. An alternative to this configuration is having a moveable lid section

108

connected to a robotic arm

80

that engages each row of chambers in a supply rack of trays

140

without ever moving the trays.

As can be understood from the above description, the sample collection system has several advantages, for example: it provides simplified prep-SFC sample collection; it collects only fractions of interest from the injected sample; it collects purified samples into removable, inexpensive, and disposable collection vials; it provides extremely efficient and controllable gas and liquid phase separation, thereby providing up to 98% consistent sample recovery; it is environmentally friendly and economical because it eliminates additional use of solvents to collect, trap, or recover samples, and clean unnecessary associated mechanical separation equipment; it allows high speed, high volume, and high purity SFC sample collection.

Because many varying and different embodiments may be made within the scope of the inventive concept herein taught, and because many modifications may be made in the embodiments herein detailed in accordance with the descriptive requirements of the law, it is to be understood that the details herein are to be interpreted as illustrative and not in a limiting sense.

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5620663	Aysta et al.	Apr 1997	A
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6183635	Klee et al.	Feb 2001	B1

Number	Date	Country
2843920	Apr 1980	DE
WO 9857181	Dec 1998	WO

Apparatus and method for preparative supercritical fluid chromatography

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Berger, Terry A: Separation of polar solutes by packed column supercritical fluid chromatography, Journal of Chromatography, A 785 (1997) 3-33.
Berger, T.A.: Packed Column SFC, The Royal Society of Chemistry 1995, pp.3-150.