Plasma lipoprotein-X quantification on filipin-stained gels: monitoring recombinant LCAT treatment ex vivo[S]

Familial LCAT deficiency (FLD) patients accumulate lipoprotein-X (LP-X), an abnormal nephrotoxic lipoprotein enriched in free cholesterol (FC). The low neutral lipid content of LP-X limits the ability to detect it after separation by lipoprotein electrophoresis and staining with Sudan Black or other neutral lipid stains. A sensitive and accurate method for quantitating LP-X would be useful to examine the relationship between plasma LP-X and renal disease progression in FLD patients and could also serve as a biomarker for monitoring recombinant human LCAT (rhLCAT) therapy. Plasma lipoproteins were separated by agarose gel electrophoresis and cathodal migrating bands corresponding to LP-X were quantified after staining with filipin, which fluoresces with FC, but not with neutral lipids. rhLCAT was incubated with FLD plasma and lipoproteins and LP-X changes were analyzed by agarose gel electrophoresis. Filipin detects synthetic LP-X quantitatively (linearity 20–200 mg/dl FC; coefficient of variation <20%) and sensitively (lower limit of quantitation <1 mg/ml FC), enabling LP-X detection in FLD, cholestatic, and even fish-eye disease patients. rhLCAT incubation with FLD plasma ex vivo reduced LP-X dose dependently, generated HDL, and decreased lipoprotein FC content. Filipin staining after agarose gel electrophoresis sensitively detects LP-X in human plasma and accurately quantifies LP-X reduction after rhLCAT incubation ex vivo.

significance of elevated LP-X in liver disease is uncertain, but it has been shown to result in xanthoma formation in cholestatic liver disease due to macrophage uptake of LP-X in the skin (14). It is important to detect LP-X in cholestatic patients, because cholestasis can present with profoundly elevated levels of plasma cholesterol (>1,000 mg/ dl) that is nonresponsive to statins or other conventional lipid-lowering therapy. Furthermore, the high levels of LP-X in cholestasis can interfere with numerous clinical laboratory tests because of turbidity issues and volume displacement from LP-X, which can lead to pseudohyponatremia and other laboratory test abnormalities (15,16).
Recently, recombinant human LCAT (rhLCAT) (ACP-501) was developed as a potential enzyme replacement therapy for FLD and for cardiovascular disease patients. It was found to be safe and well-tolerated in a phase I clinical trial (17). Infusion into a patient with FLD also showed promising results: HDL-C rapidly increased, peaking to nearly normal levels in 8-12 h (18). Importantly, anemia improved and renal function stabilized after long-term treatment with ACP-501 (18). This trial demonstrated that enzyme replacement therapy with rhLCAT is a potential strategy for increasing HDL-C in FLD; however, the effect of rhLCAT on LP-X was not examined. Moreover, relatively high levels of ACP-501 were required to raise HDL to nearnormal levels in this study. After completion of this study, a more potent formulation of rhLCAT, MEDI6012, with a longer half-life was developed and is now being tested in patients with cardiovascular disease in a phase II clinical trial (19).
A validated rapid clinical method for measuring plasma LP-X levels would be useful not only for identifying patients with LP-X that could potentially benefit from rhL-CAT treatment, but also for monitoring LP-X levels during rhLCAT therapy for FLD. Currently, however, there are no routinely available assays for efficient screening for LP-X in patient plasma. Agarose gel electrophoretic analysis of patient plasma has shown that LP-X particles migrate toward the cathode, i.e., with reverse electrophoretic mobility compared with other lipoproteins (13). LP-X, however, is difficult to detect using Sudan Black or other similar neutral lipid stains that are typically used to stain lipoproteins separated by gel electrophoresis. In contrast to normal plasma lipoproteins, which are enriched in neutral lipids (CEs and triglycerides), LP-X particles are deficient in neutral lipids and instead, as noted above, are highly enriched in FC and phospholipids (1).
Filipin, a fluorescent polyene antibiotic, binds specifically to FC. In contrast to Sudan Black, it does not stain neutral lipids. It is widely used as a cytochemical fluorescent stain for FC, but also has been used to detect FC in normal lipoproteins in nondenaturing polyacrylamide gels (20).
In this work, we demonstrate that filipin staining of agarose gels after electrophoresis is a relatively easy and sensitive method to detect and quantitate LP-X in plasma from FLD and cholestasis patients. It can also be used to monitor the effects of exogenous rhLCAT on lipoproteins. Finally, our new methodology presents a potential opportunity, at both the clinical and basic science level, to investigate the relationships between FC-enriched lipoproteins and LP-X in the pathology of FLD and cholestatic liver disease.

Preparation of synthetic LP-X
Synthetic LP-X, which was used as a calibrator and to examine the differential staining of FC by filipin and Sudan Black, was prepared as described in Ossoli et al. (8), with minor modifications. Briefly, multilamellar LP-X particles containing 24 mol% cholesterol were formed by combining 24.4 mg L--lecithin (Avanti Polar Lipids, Inc., Alabaster, AL) with 4.25 mg cholesterol (Sigma Chemicals, St. Louis, MO) from their respective stock solutions in chloroform and then drying the lipid mixtures under nitrogen. Two milliliters of normal saline were added to the dried lipids and the mixture was vortexed and sonicated as described in Ossoli et al. (8) to generate multilamellar particles enriched in FC and phospholipid in the typical size range of LP-X.

Agarose gel electrophoresis
Synthetic LP-X (10 µl) or EDTA-plasma (10 µl) was loaded on Sebia Hydragel 15/30 lipoprotein (e) agarose gels (#4134; Sebia, Inc., Norcross, GA). Purified lipoproteins (LDL, VLDL, and HDL) were loaded on the same gel. Electrophoresis was for 1 h at 100 V in barbital buffer (#B5934-12VL; MilliporeSigma, St. Louis, MO) in a Titan gel electrophoresis chamber (Helena Laboratories, Beaumont, TX). Gels were either fixed and stained with Sudan Black to detect neutral lipids, according to the manufacturer's instructions, or incubated with filipin stain to detect FC by a modification of the method described in (20). Filipin stain was prepared fresh each time by dissolving 50 mg of filipin (Polysciences, Inc., Warrington, PA) in 2.0 ml N,N′-dimethylformamide, and then adding 100 ml 1× PBS containing 0.1% sodium azide and mixing thoroughly. Filipin and filipin-containing solutions were shielded from light at all stages, as filipin is light sensitive. Immediately after electrophoresis, gels were washed for 5 min in 1× PBS plus 0.1% sodium azide and then incubated overnight in 30 ml of filipin stain at 4°C with gentle rocking, shielded from light. Gels, kept in the dark at all times, were then washed for 10 min at room temperature, then again for 1 h with 100 ml of wash solution (1× PBS). Fresh wash solution was added 10 min before imaging. Gels were placed on the AlphaImager's UV light transilluminator (Pro-teinSimple, San Jose, CA) and photographed using the ethidium bromide filter, similar to photographing an ethidium bromidestained DNA gel. LP-X, which migrates toward the cathode in the opposite direction as normal lipoproteins, was quantified by densitometry (including the origin) and background in an equalsized area of the gel 1 cm below the bottom of each band was subtracted using AlphaImager software. To ensure linearity of the filipin signal, multiple exposures were taken of gels and quantitation was performed only on exposures in which band intensities did not reach saturation, as determined by the AlphaImager software. Supplemental Fig. S1 demonstrates that the UV light exposures used to visualize filipin on our gels do not result in photobleaching.

Subjects
This study was approved by the National Heart, Lung, and Blood Institute, Institute Review Board (protocol 03-H-0280) and is compliant with the Declaration of Helsinki principles. All subjects provided informed consent prior to participation in the study.

Plasma collection and incubation with rhLCAT
EDTA-plasma was collected from patients (FLD, FED, or cholestasis) and stored on ice or at 4°C until electrophoresis. Precision studies for LP-X in FLD patient plasma are described in supplemental Fig. S2. rhLCAT (MEDI6012) was produced as described before (21) and was kindly provided by MedImmune. Fresh never-frozen FLD plasma was incubated at 37°C overnight with MEDI6012 (0-1,000 ug/ml) and aliquots were analyzed for lipids (Cholesterol-E and Free Cholesterol-E; Wako Diagnostics, Mountain View, CA) and for lipoproteins and LP-X by agarose electrophoresis followed by Sudan Black or filipin staining.

Depletion of apoB-Lps from FLD plasma
EDTA-plasma was collected as described above and incubated with dextran sulfate or LipoSep IP™ (Sun Diagnostics, New Gloucester, ME), following the methodology of Davidson et al. (22). Briefly, in the dextran sulfate method, 2.0 µl of 5% dextran sulfate (molecular weight 500,000) and 5.0 µl of 1 M MgCl 2 were added to 100 µl of FLD patient plasma. The mixture was incubated for 20 min at room temperature and then centrifuged at 3,000 g for 10 min. For depletion of apoB-Lps using the LipoSep IP™ reagent, FLD patient plasma was combined with an equal volume of the LipoSep IP™ reagent in a 1.5 ml microcentrifuge tube and immediately vortexed at top speed. The mixture was incubated at room temperature for 10 min and then centrifuged at 12,000 g at 4°C for 10 min. The supernatant, consisting of apoBdepleted plasma, was used immediately for agarose gel electrophoresis, and the pellet was discarded.

Statistical analysis
Statistical analyses were performed using GraphPad Prism. To fit the allosteric curve of LP-X versus FC concentration during MEDI6012 incubation (Fig. 4C), the "Agonist vs. Response-Variable Slope, 4 parameters" equation under "Dose-Response Curve-Stimulation" in GraphPad Prism was applied to the data. The concentration of MEDI6012 required to decrease LP-X by 50% in Fig. 4D was determined by analyzing the data in GraphPad Prism similar to determining the "IC50" of MEDI6012 [nonlinear regression, enzyme kinetics (inhibitor) vs. response analysis]. Unless otherwise indicated, all results are presented as the mean ± 1 SD.

Filipin, but not Sudan Black, quantitatively stains cholesterol on LP-X
Synthetic LP-X was prepared in vitro from purified FC and phosphatidylcholine and various dilutions (0.2-200 mg/dl cholesterol) were subjected to electrophoresis on duplicate agarose gels, which were then stained with either filipin to detect FC or Sudan Black to detect neutral lipids. Figure 1A shows that synthetic LP-X migrates from the origin (horizontal red line) toward the cathode, as expected, opposite to LDL, VLDL, and HDL, which migrate in the traditional lipoprotein direction toward the anode. Moreover, filipin, but not Sudan Black, stains synthetic LP-X Fig. 1. Filipin staining of synthetic LP-X after agarose gel electrophoresis. A: Filipin, but not Sudan Black, stains synthetic LP-X. Sequential dilutions of synthetic LP-X (10 µl), corresponding to 200, 80, 40, 20, 10, 4, 2, 0.8, 0.4, and 0.2 mg/dl FC, were loaded into lanes 1-10, respectively, of two identical gels, and the gels were run at 100 V for 1 h. The gels were stained with either filipin (left) or Sudan Black (right). LDL, VLDL, HDL, and healthy control (HC) plasma (10 µl) were included as standards loaded on the left side of each gel and the red line indicates the position of the origin (ORI) (application point). LP-X can be seen as fluorescent material migrating toward the cathode ("backward-running" compared with LDL, VLDL, and HDL) by filipin staining, but it is undetectable on gels stained with Sudan Black. B: LP-X fluorescence on agarose gels is proportional to the amount of LP-X FC loaded on the gels. Three identical gels similar to A but with 200, 133, 100, 56, 40, 26.7, and 20 mg/dl FC were run and stained with filipin as above. Lp-X fluorescence for each sample was quantitated by densitometric analysis and the average and SD for each point was graphed versus the amount of LP-X FC loaded. Linear regression analysis using Prism revealed linearity over an order of magnitude, with R 2 = 0.9855 (Fig. 1A). The lowest observable amount of synthetic LP-X that could be visualized with filipin was approximately 1 mg/dl FC (Fig. 1A). In Fig. 1B, LP-X dilutions between 20 and 200 mg/dl were run on triplicate agarose gels and stained with filipin for a precision study. Densitometry demonstrated that the relationship is linear between 20 and 200 mg/dl LP-X cholesterol, with R 2 of 0.9855 (Fig.  1B). The inter-assay coefficient of variation for quantifying the cholesterol content of LP-X was less than 12% across the concentration range tested.

Filipin, but not Sudan Black, sensitively detects LP-X in plasma from FLD and cholestatic patients
Fresh, never-frozen plasma from FLD patients was subjected to electrophoresis on agarose gels followed by staining with either filipin or Sudan Black ( Fig. 2A, B). Figure  2A shows a patient ("FLD1") with very high levels of LP-X that was readily detectable as a broad filipin-stained band below the origin (migration toward the cathode). Only a faint band, however, could be seen after Sudan Black staining, indicating that detection of LP-X by filipin staining is much more sensitive than Sudan Black. Moreover, compared with the normolipidemic sample (healthy control) there was increased filipin staining in the FLD sample in the LDL region, migrating toward the anode. As can be seen below in the other FLD samples tested, this was a common finding. We found that immunodepleting apoB-Lps with the LipoSep IP™ reagent (22) removed essentially all filipin-stained -migrating lipoproteins (supplemental Fig.  S3), demonstrating that apoB-Lps are indeed FC-enriched in FLD patients and are almost exclusively responsible for filipin staining in and around the LDL region of the gel. We also frequently noted that the purified lipoprotein standards (LDL, VLDL, and HDL) that are isolated by density gradient ultracentrifugation from normolipidemic samples all stain with Sudan Black, but only LDL and VLDL stain well with filipin. Figure 2B shows the results from two cousins with FLD. The patient on the left ("FLD2") had more LP-X by filipin staining, and also more advanced renal disease, than the patient shown on the right ("FLD3"). However, only an extremely faint LP-X band migrating in the cathodal direction could be observed for both FLD2 and FLD3 after staining with Sudan Black, again showing the increased sensitivity for LP-X detection by filipin staining. As can be seen in patient FLD2, we sometimes observe in FLD patients a filipin-stained band at the origin, which may be large LP-X that cannot migrate into the gel. Figure 2C demonstrates that filipin staining is so sensitive that it can even detect very low levels of LP-X in an FED patient. FED patients have low HDL-C and corneal opacities, but do not develop renal disease. Until now, LP-X has not been reported in FED patients, and the absence of LP-X was thought to be the explanation for why they do not develop renal disease (1). The increased sensitivity of filipin staining appears to allow the detection of even extremely low levels of LP-X that are below the threshold for the development of renal dysfunction. Precision studies for LP-X in FLD patient plasma are described in supplemental Fig. S2. Figure 2D shows LP-X in a patient with cholestasis from graft-versus-host disease. In general, we have observed that cholestatic LP-X is present in plasma at much higher levels than in FLD plasma, as determined by filipin staining and, as in this case, can often be detected by Sudan Black staining as well.

Freezing and thawing of samples interferes with LP-X detection
In Fig. 3, the stability of LP-X detection to freezing and thawing was investigated. Synthetic LP-X (lanes 1-4) or plasma from an FLD patient (lanes 5-8) were either maintained at 4°C without freezing or freeze-thawed one, two, or three times. Synthetic LP-X maintained at 4°C (lane 1, filipin-stained gel) migrated as a smear toward the cathode, but after just a single freeze-thaw (lane 2), synthetic LP-X was no longer detectable by filipin staining. Similarly, in FLD plasma, a cathode-migrating LP-X band seen by filipin staining in the nonfrozen sample (lane 5, filipin-stained gel) could not be observed after a single freeze-thaw (lane 6, filipin-stained gel). In addition, the filipin intensity at the origin was also diminished after just a single freezethaw. The overall level of filipin staining of all lipoprotein fractions was decreased by further freeze-thawing (lanes 7 and 8, filipin-stained gel). Consistent with our previous results, neither synthetic LP-X nor backward-running LP-X in FLD patient plasma was stained by Sudan Black (lanes 1-8, Sudan Black-stained gel). Sudan Black-stained FLD lipoproteins with LDL mobility were somewhat diminished after the first freeze-thaw, but not by subsequent freezethaws (lanes 5-8, Sudan Black-stained gel). The filipinstained gels clearly demonstrate that freezing and thawing interferes with LP-X detection.

Incubation of FLD plasma with rhLCAT decreases LP-X in a dose-dependent manner
To investigate the ex vivo effects of rhLCAT (MEDI6012) on LP-X in plasma, increasing doses of MEDI6012 were incubated with plasma from an FLD patient ("FLD4"). Figure  4A shows that FC decreased and CEs increased with increasing doses of MEDI6012. Consistently, MEDI6012 decreased LP-X and increased HDL on agarose gels stained with filipin and Sudan Black, respectively, for the proband (Fig. 4B). Figure 4C demonstrates a strong correlation between LP-X and FC at different doses of MEDI6012, with both FC and LP-X diminishing with increased doses of MEDI6012. Interestingly, the relationship between FC and LP-X during the course of MEDI6012 incubation was not linear, but instead appeared to be allosteric (Fig. 4C), with decreased efficiency of FC esterification occurring after an 4-fold drop in LP-X, from 8,000 to 2,000 (corresponding to 10 ug/ml MEDI6012). This allosteric relationship suggests that structural changes to LP-X occurring past this point may affect the efficiency of FC esterification. Figure 4D indicates that the dose of MEDI6012 required to decrease LP-X by half in this in vitro assay is approximately 3.7 ug/ml.

DISCUSSION
The main advance in this study was the development of a sensitive, reliable filipin gel-based assay for the detection and quantitation of plasma LP-X. Using this assay, we also made several potentially important findings related to lipoprotein abnormalities in FLD and have explored the feasibility of using LP-X as a biomarker for monitoring rhLCAT therapy.
As is readily apparent, the positive staining of synthetic LP-X with filipin but absence of staining with Sudan Black indicates that detecting endogenous plasma LP-X with filipin should be more sensitive compared with Sudan Black. It varies depending on the lipoprotein class, but normal lipoproteins typically contain neutral lipids as their major component (23) and, hence, readily stain with Sudan Black. In contrast, LP-X contains less than 10% neutral lipids (1,24). This probably accounts for our past inability to detect LP-X in many of our FLD patients when stained with Sudan Black. It is likely that only in those patients with very high levels of LP-X is it possible to detect LP-X with Sudan Black. The increased sensitivity of our method also probably accounts for the detection of LP-X in our one FED patient. Additional FED patients need to be examined, but it may be that low levels of LP-X are often present in FED patients, but are below the level at which nephrotoxicity is observed.
Regardless of the staining method used, a key to detecting LP-X by electrophoresis is its "backward" or cathodal migration. Normally, lipoproteins contain a net negative charge, most likely because of their protein content, and hence migrate toward the anode. We observed that not only endogenous LP-X from our FLD patients but also synthetic LP-X migrated toward the cathode. The synthetic LP-X was made with phosphatidylcholine, a zwitterion, and Fig. 3. LP-X is unstable to freezing and thawing. Synthetic LP-X (lanes 1-4) or FLD plasma (lanes 5-8) was either maintained at 4°C (lanes 1 and 5) or freezethawed one time, two times, or three times (lanes 2, 3, and 4 for synthetic LP-X and lanes 6, 7, and 8 for FLD, respectively). Samples were frozen at 70°C for at least 16 h before each thaw. Electrophoresis and staining was as described in Fig. 1. thus has no net charge. Endogenous LP-X is relatively devoid of proteins and, based on its lipid composition (1), does not appear to be enriched in cationic lipids. The backward migration of LP-X is, therefore, most likely due to electroendosmosis (25,26), which causes the bulk movement of buffer ions that nonspecifically sweeps neutrally charged particles toward the cathode. Besides charge, agarose gel electrophoresis also separates lipoproteins based on their size. Large lipoproteins move more slowly relative to smaller particles, which explains why chylomicrons typically get trapped at the origin (application point). We also observed filipin-stained bands in fasted samples at the origin in some of our FLD patients. It is known that LP-X can be quite heterogenous in size (24,26) and, thus, some LP-X particles can perhaps be too large to enter the gel. Because the filipin-enriched bands migrating at the origin were still present after immunodepletion of apoB-Lps, and synthetic LP-X also contained a subpopulation of filipinstained particles that remained at the origin, the filipinstained material remaining at the origin in patient plasma is most likely LP-X. Size heterogeneity could also account for the fuzzy bands and smearing in the migration position for LP-X that we observed in our FLD patients or with our synthetic LP-X particles. Finally, cholestatic patient plasma had significant Sudan Black staining of backward-running LP-X. Whether the exact migration position of LP-X has any disease relevance is not known at this time, but can be examined in the future with our assay.
Another observation that we made based on filipin staining is that there is enrichment of FC in FLD patients not only in LP-X but also in and around the "" region where LDL typically migrates on agarose gels and sometimes almost as far as VLDL. Supplemental Fig. S3 demonstrates that immunodepleting apoB-Lps removes almost all filipin staining in this "broad-" region, confirming that these FC-enriched bands do in fact correspond to apoB-Lps. This is consistent with the known chemical composition of apoBcontaining lipoproteins from FLD patients, which have higher levels of FC (6). VLDL has also been reported to migrate as -lipoproteins in FLD (6). Whether these abnormal lipoprotein particles may also impact on the pathogenesis of FLD is not known, but cholesterol enrichment of lipoproteins in SR-BI-KO mice has been shown to lead to abnormal red cell shape changes, which also occur in FLD, and to enrichment of cholesterol in platelets and their hypercoagulability (27). Although LP-X is relatively devoid Fig. 4. MEDI6012 incubation with FLD patient plasma. A: Lipids of FLD patient plasma treated with MEDI6012 ex vivo. FLD plasma was incubated with increasing doses (0, 0.75, 1.5, 3, 10, 30, 100, 300, and 1,000 ug) of MEDI6012 per milliliter of plasma at 37°C for 16 h and total cholesterol and FC were measured. CE was calculated as the difference between total cholesterol and FC. Green lines and yellow lines with blue-circled dots represent total cholesterol and FC, respectively, in milligrams per deciliter. Orange and red lines represent percent FC and CE remaining after MEDI6012 incubation, using plasma levels at 0 mg/ml MEDI6012 as 100%. B: LP-X disappears and HDL appears after MEDI6012 incubation with FLD patient plasma. Lanes 1-9 represent doses, 0, 0.75, 1.5, 3, 10, 30, 100, 300, and 1,000 ug/ml, respectively, of MEDI6012. The leftmost 4°C sample was FLD patient plasma drawn fresh the day of electrophoresis and maintained at 4°C until applied to the gel. The 4°C sample to the right of that was from the same blood draw as the MEDI6012-incubated samples, but was kept at 4°C overnight without MEDI6012 as a control, while the experimental samples from the same blood draw were incubating at 37°C overnight. Electrophoresis and staining with filipin (left) or Sudan Black (right) were as described in Fig. 1. C: Plasma LP-X correlates with levels of FC in plasma after MEDI6012 incubation. Cathode-migrating LP-X in lanes 1-9 of B (corresponding to 0-1,000 ug/ml MEDI6012 of the filipin-stained gel) was quantitated by densitometry and plotted against the corresponding plasma FC for each sample after MEDI6012 incubation. The "0 ug/ml" dose of MEDI6012 had the highest levels of LP-X and FC in plasma, and the "1,000 ug/ml" dose had the lowest LP-X and FC levels. D: The concentration of MEDI6012 required to decrease LP-X halfway between the highest and lowest LP-X values (similar to an IC50 analysis) was determined using GraphPad Prism. of proteins, they have been reported to bind apoC-class proteins (1,24), which have a negative charge (28). Supplemental Fig. S4 demonstrates that adding purified apoC-II to synthetic LP-X in vitro decreases cathodal LP-X migration on agarose gels. In fact, at very high ratios of apoC-II to synthetic LP-X, a subpopulation of LP-X particles can be seen to migrate toward the anode, with mobility in the LDL/VLDL region. Incorporation of negatively charged lipids, such as free fatty acids, into LP-X particles can also cause the particles to migrate toward the anode (29). Thus, some of the filipin-stained particles migrating with  mobility, particularly those with LP-X-like instability to freezing and thawing, might also be LP-X.
A limitation of our assay is that frozen plasma samples do not appear to be suitable for analysis. Unlike normal lipoproteins that have a micellar-like structure of surface phospholipids and FC, with a neutral lipid core, LP-X is thought to be a multi-lamellar vesicle made of phospholipid and FC. It is thought to have an aqueous core made up of nonspecifically trapped plasma proteins. It is therefore likely that freezing of LP-X causes a disruption of its structure when ice crystals form in the aqueous core. If so, it may be possible to preserve LP-X to freezing by adding a cryoprotectant, as has been done before for preserving lipoproteins (30,31). We also observed, however, a general decrease in total filipin staining after freezing and thawing. Possibly the lipids have reorganized after freezing, decreasing the ability of filipin to interact with cholesterol, which may not be prevented even in the presence of cryoprotectant.
Because of the necessity of having a fresh sample and the rarity of FLD, we have only analyzed a limited number of samples by our new method. More studies will be needed to determine whether quantitation of the cholesterol content of LP-X, which we showed is possible with our assay, can be used to predict risk for renal disease. In the case of cholestasis, the filipin-gel staining method could be useful to determine the extent of cholesterol on LP-X versus other lipoproteins, which may be predictive of their response to lipid-lowering therapy. The ex-vivo recombinant LCAT spiking studies into FLD plasma are promising and suggest that this method may also be useful in determining the response to rhLCAT therapy in FLD patients. Interestingly, the dose that caused almost the complete dissolution of LP-X is in the physiologic range and is similar to what was used in phase 2a clinical trials of rhLCAT (19). The generation of CEs by the added rhLCAT in our study must cause a spontaneous reorganization of the LP-X particles. We even observed the in vitro formation of HDL, which again must occur after rhLCAT forms CEs, allowing the residual apoA-I in the plasma from FLD patients to form HDL-like particles.
In conclusion, filipin staining of agarose gels can be used to detect and quantitate LP-X from FLD plasma and cholestasis. This novel methodology addresses an important deficiency in the measurement of LP-X and has several potential clinical and basic science applications.