Abstract

We succeeded in developing the fingerprint of natural product by eastern blotting using monoclonal antibodies. After developing and separating them on a TLC plate, solasodine glycosides are oxidized by NaIO4 and reacted with a protein to give conjugates which are recognized with anti-solamargine monoclonal antibody (MAb). Anti-solamargine MAb having wide cross-reactivity can stain and detect all solasodine glycosides by fingerprint. Different sensitivity between solamargine and solasonine was observed. The detection limit was 1.6 ng of solasonine. The hydrolysed products of solamargine were determined by fingerprint of eastern blotting compared to their Rf values depending on the sugar number. Fingerprint by eastern blotting using anti-ginsenoside Rb1 MAb distinguished the formula containing ginseng prescribed in traditional Chinese medicine. By double-staining of ginsenosides it is possible to suggest that the staining color shows the pharmacological activity, such as the purple bands indicate ginsenosides having stimulation activity, and the blue color indicated compound like ginsenosides possessed the depression affect for the central nervous system (CNS), respectively.

1. Introduction

In the recent rapid development of the molecular biosciences and their biotechnological applications, immunoassay systems using monoclonal antibody (MAb) against drugs and small molecular weight bioactive compounds have become an important tool for studies on receptor binding analysis, enzyme assay, and quantitative and/or qualitative analytical techniques in animals or plants; owing to their specific affinity. Previously we prepared various kinds of MAb against natural products like forskolin [1], solamargine [2], crocin [3], marihuana compound [4], opium alkaloids [5], ginsenosides [6, 7], berberine [8], sennosides [9], paeoniflorin [10], glycyrrhizin [11, 12], ginkgolic acid [13], aconitine alkaloid [14], baicalin [15], and so on, and developed individual competitive enzyme-linked immunosorbent assay (ELISA) as a high sensitive, specific, and simple methodology.

Western blotting is widely used as an immunostaining technique to detect high-molecular compounds like peptides and proteins based upon an antigen-antibody reaction. However, low-weight molecular compounds had not been previously analyzed by western blotting. We succeeded the blotted staining of solasodine glycoside on PVDF membrane using MAb after developed and separated solasodine glycosides on TLC and called as new-western blotting [16]. From this evidence, we applied this new methodology to licorice glycoside, glycyrrhizin, and named it as eastern blotting [12] following ginsenosides [1719] and saikosaponin [20], and so on. In this paper, we introduce the fingerprint of a steroidal alkaloid glycoside, solasodine glycoside and ginseng saponin, ginsenosides by eastern blotting using MAbs.

2. Materials and Methods

2.1. Preparation of Anti-Solamargine MAb

A hybridoma producing MAb reactive to solamargine was obtained by the general procedure in our laboratory and classified into IgG2b which had k light chains [2]. The reactivity of IgG type MAb, SMG-BD9, was tested by varying antibody concentration and by performing a dilution curve. The antibody concentration was selected for competitive ELISA. The MAb following competition was bound to polystyrene microtiter plates precoated with solamargine HSA. Under these conditions, the full measuring range of the assay extended from 20 to 400 ng/mL [2].

Anti-ginsenoside Rb1 [6] and Rg1 [7] were also prepared by the same ways in our laboratory.

2.2. Fingerprint by Eastern Blotting [16]

Solasodine glycosides were developed on a TLC plate. The TLC plate was covered with the PVDF membrane and blotted by short heating. The blotted PVDF membrane was dipped in water containing NaIO4 under stirring at room temperature for 1 hr. After washing with water, a carbonate buffer containing BSA was added and stirred at room temperature for 3 hr. The PVDF membrane was washed twice with phosphate buffer for 5 min, and then washed with water. The PVDF membrane was immersed in anti-solamargine MAb, stirred at room temperature for 1 hr. After washing the PVDF membrane twice with phosphate buffer and water, a 1000-fold dilution of peroxidase-labeled goat anti-mouse IgG in phosphate buffer (pH 7.2) was added and stirred at room temperature for 1 hr. The PVDF membrane was washed twice with phosphate buffer and water, then exposed to 4-choloro-1-naphthol (1 mg/mL)—H2O2 (0.03%) in phosphate buffer (pH 7.2), and eastern blotting was stopped by washing with water. The immunostained PVDF membrane was allowed to dry.

2.3. Hydrolysis of Solasodine Glycosides and Stained by H2SO4, Dragendorff, and Eastern Blotting

Solamargine and solasonine were hydrolyzed by using 1 M HCl and heated for 10, 20, 30, 60, and 90 minutes, respectively. The hydrolyzed products were applied on three silica gel TLC plates. Developments were made by using CHCl3/MeOH/NH4OH (7 : 2.5 : 1) as mobile phase. Two plates were sprayed with H2SO4 and Dragendorff reagent, respectively. But the third TLC plate was transferred to a PVDF membrane by heating and stained as indicated above.

3. Results and Discussion

3.1. Fingerprint of Solasodine Glycosides by Eastern Blotting

The natural resources of adrenocortical hormones and sex hormones, which are mainly obtained from diosgenin, are becoming rare. The most important feature of solasodine is that it can be converted to dehydropregnenolone. Solasodine is found with a series of sugar residues attached to the oxygen at the C-3 position. By far the most common forms are the triglycosides, solamargine being predominant. Therefore, the steroidal alkaloid glycosides of the solasodine type like solamargine have become important as a starting material for the production of steroidal hormones in the pharmaceutical and medicinal areas. Rapid, simple, highly sensitive, and reproducible assay systems are required for a large number of plants, and a limited small amount of samples. In order to select the strain of higher yielding steroidal alkaloid glycosides in the resources of Solanum species we prepared an anti-solamargine MAb which was unique having a wide cross-reactivity [2].

Clear blue spots appeared on PVDF membrane as shown in Figure 1, the immunostains of solamargine and solasonine were observed. Lane 1–5 demonstrated the concentrations of both alkaloids, 0.8, 1.6, 8, 40, and 200 ng, respectively. Different sensitivities between solamargine and solasonine were observed in individual concentrations, and the sensitivity of solasonine was somewhat higher than that of solamargine. The detection limit was 1.6 ng of solasonine. We succeeded to separate the function of small molecule compounds such as solasodine glycosides into a part of epitope and fixing on the membrane [16]. When glycosides are treated by NaIO4, the sugar part is cleaved to release an aldehyde group which is prepared a Schiff base with protein and then fixed to PVDF membrane. On the other hand, an epitope can be detected by MAb as described in Figure 2.

In order to confirm the preparation of solamargine-BSA conjugate on the PVDF membrane, the band corresponding to the solamargine-BSA conjugate was assessed by MALDI mass spectrometry. A broad peak [M+H]+ of solamargine-BSA conjugate appeared at around m/z 69043 in MALDI mass spectrometry demonstrating that at least 1-2 molecules of solamargine had combined [6] (data not shown). Therefore, it became clear that the sugar moiety which was conjugated with BSA is necessary in this staining system. Moreover, we confirmed the above evidence that solasodine glycoside-protein conjugate is necessary for the eastern blotting because solasodine which has no sugar moiety in a molecule cannot be stained by eastern blotting although solasodine can be stained by H2SO4 and Dragendorff reagent (see Figures 3(b) and 3(c)).

As an application of finger printing by newly established eastern blotting, the hydrolysis pathway of solamargine was surveyed by eastern blotting using anti-solamargine MAb. Solamargine was hydrolyzed using 1 M HCl for 10, 20, 30, 60, and 90 minutes, respectively. The hydrolyzed products were developed by three silica gel TLC plates using CHCl3/MeOH/NH4OH solvent system. Two plates were sprayed and colored with H2SO4 and Dragendorff reagent, individually. One TLC plate was blotted to a PVDF membrane and stained by eastern blotting. Clear blue spots appeared as shown in Figure 3. Figure 3(a) shows the eastern blotting of solasodine glycosides. Lanes 1–6 demonstrate solamargine, 10, 20, 30, 60, and 90 minutes hydrolyzed products, individually, solasodine, 3-O-β-D-glucopyranosyl solasodine, L-rhamnosyl-(1-4)-O-3-β-D-glucopyranosyl solasodine, L-rhamnosyl-(1-2)-O-3-β-D-glucopyranosyl solasodine, and solamargine, respectively. This fingerprinting phenomenon agreed with the structural confirmation of solasodine glycosides elucidated by 13C NMR [21]. When compared with the sensitivity of fingerprinting regarding solasodine glycosides, the eastern blotting was more sensitive than those stained by H2SO4 (Figure 3(b)) and Dragendorff (Figure 3(c)).

We also analyzed the fingerprinting of Solanum species as shown in Figure 4. The profile stained by H2SO4 (Figure 4(b)) indicated the complicated pattern which is not limited to solasodine glycosides compared to the eastern blotting profile (Figure 4(a)). Major solasodine glycoside are solasonine, solamargine, and khasianine as indicated in Figure 4. From the survey of solasodine glycoside we decided that S. khasianum is an important resource of adrenocortical hormones and sex hormones.

Moreover, we succeeded to breed the strain of higher yielding solasodine glycoside by inducing the single chain Fv gene cloned from anti-solamargine MAb into Solanum khasianum plant [22].

3.2. Fingerprint of Ginseng Saponin, Ginsenoside, by Eastern Blotting

Ginseng, the crude drug of Panax ginseng is one of the most important natural medicine in many countries. It has been used to enhance stamina and capacity to cope with fatigue and physical stress, and as a tonic against cancers, disturbances of the central nervous system (CNS), hypothermia, carbohydrate and lipid metabolism, immune function, the cardiovascular system, and radioprotection [23]. They contain more than 50 kinds of dammarane and oleanane saponins considered to be pharmacologically active components. Ginsenoside Rb1 is a main saponin in ginseng. However, since the concentration varies in the ginseng root or the root extract depending on the method of extraction, subsequent treatment, or even the season of its collection, standardization of quality is required. For this purpose we have prepared anti-ginsenoside Rb1 [6] and Rg1 MAbs [7].

Cross-reactivity is the most important factor in determining the value of an antibody. Since the ELISA for ginsenoside Rb1 was established for phytochemical investigations involving crude plant extract, the assay specificity was checked by determining the cross-reactivity of the MAb with various related compounds. The cross-reactivity data of MAb that was obtained were examined by competitive ELISA and calculated using picomole of ginsenoside Rb1. The cross-reactivity of ginsenoside Rc and Rd which possess a diglucose moiety attached to the C-3 hydroxy group were weak compared to ginsenoside Rb1, 0.024 and 0.020%, respectively. Ginsenoside Re and Rg1 showed no cross-reactivity (less than 0.005%). It is evident that the MAb reacted only with a small number of structurally related ginsenoside Rb1 molecules very weakly and did not react with other steroidal compounds like glycyrrhizin, digitoxin, tigogenin, tigonin, and solamargine. Anti-ginsenoside Rg1 MAb [7] and Re [18] have been prepared and set up their ELISA. Anti-ginsenoside Rg1 MAb was also high specific like anti-ginsenoside Rb1. On the other hand, anti-ginsenoside Re MAb showed wide cross-reactivity. Therefore, this MAb can be used for the analysis for the total ginsenoside concentration.

Figure 5 shows the H2SO4 staining and eastern blotting of ginsenoside standards and the traditional Chinese medicine (TCM) using anti-ginsenoside Rb1 MAb. It is impossible to determine the ginsenosides by TLC-staining by H2SO4 as indicated in Figure 5(a). On the other hand, clear staining of ginsenoside Rb1 occurred by eastern blotting (Figure 5(b)). Furthermore, it became evident that kikyoto and daiokanzoto prescriptions related to TCM prescription that did not contain ginseng indicating no band of ginsenoside Rb1. The eastern blotting method was considerably more sensitive than that of H2SO4 staining. The H2SO4 staining detected all standard compounds. The Eastern blotting indicated only limited staining of ginsenoside Rb1, Rc, and Rd, of which cross-reactivities were under 0.02%. We suggest that an aglycon, protopanaxadiol, and a part of the sugars may be of importance to the immunization and may function as an epitopes for the structure of ginsenosides. In addition, it is suggested that the specific reactivity of sugar moiety in the ginsenoside molecule against anti-ginsenoside Rb1 MAb may be modified by the NaIO4 treatment of ginsenosides on the PVDF membrane causing ginsenoside Rc and Rd to become detectable by eastern blotting.

When the mixture of anti-ginsenoside Rb1 and Rg1 MAbs and the pair of substrates were tested for staining of ginsenosides, all ginsenosides, ginsenoside-Rb1, -Rc,-Rd,-Re, and -Rg1 were stained blue although the purple color staining for ginsenoside Rg1 was expected because 3-amino-9-ethylcarbazole and 4-chloro-1-naphotol might be different. Therefore, we performed successive staining of the membrane using anti-ginsenoside Rg1 and then anti-ginsenoside Rb1. Finally, we succeeded: the double-staining of ginsenosides indicating that ginsenoside Rg1 and ginsenoside Re were stained purple and the other blue, as indicated in Figure 6. From this result, both antibodies can distinguish individual aglycon protopanaxatriol and protopanaxadiol. For this application, the crude extract of various Panax species were analyzed by the newly developed double-staining system. Major ginsenosides can be determined clearly by the double staining method indicated in Figure 6 as the fingerprint of ginsenosides. Therefore, it is possible to suggest that the staining color shows the pharmacological activity, such as the purple bands indicate ginsenosides having stimulation activity for the CNS. On the other hand, the blue color indicates ginsenosides possessing the depression affect for the CNS. Moreover, the Rf value of ginsenosides roughly suggests the number of sugars attached to the aglycon. Both analyses make it possible to identify which aglycon attaches and how many sugars combine, leading to the structure of ginsenosides. In fact, three kinds of ginsenosides possessing protopanaxadiol-ginsenoside Rh1, Rf, and 20-O-gluco-ginsenoside Rf in P. ginseng root were determined by coloring and Rf value by comparing them with the structures reported in the previous paper [19].

4. Conclusion

Fingerprint by eastern blotting method can open its application for the wide field of natural products, especially glycosides like solasodine glycosides and ginsenosides. An MAb having a wide cross-reactivity like anti-solamargine MAb can distinguish the total solasodine glycosides. On the other hand, a high specific MAb like anti-ginsenoside Rb1 MAb can be used for the detection of a single antigen compound.

When two kinds of MAbs can be used, the double-staining is possible as the staining system enhanced the separate staining of ginsenosides having protopanatriol or protopanaxadiol in a molecule. The staining color can monitor the pharmacological activity suggesting the stimulation activity and/or the depression affect for the CNS. Furthermore, the Rf value of solasodine glycosides and ginsenosides suggests the number of sugars attached to the aglycon. Both evidences make it possible to confirm which aglycon attaches and how many sugars combine to the aglycon resulting the confirmation of structure for glycosides. Therefore, the fingerprint stained by eastern blotting using MAb could provide a new strong methodology in the wide field of natural product investigation.