The structures and MDR ratios of 35 purine derivatives in the training/test sets.
1. Introduction
Therapy for central nervous system (CNS) diseases requires drugs that can cross the blood-brain barrier (BBB) (Cheng et al, 2010). BBB not only maintains the homeostasis of the CNS, but also refuses many potentially important diagnostic and therapeutic agents from entering into the brain (Chen et al, 2009). The pathogenesis of Alzheimer's disease (AD) senile plaque and neurofibrillary tangle lesions putatively involves a compromised BBB (Jevnes & Provias, 2011), which protects the brain against endogenous and exogenous compounds and plays an important part in the maintenance of the microenvironment of the brain (Vogelgesang et al, 2011). The ability of drug permeating across BBB becomes critical in the development of new medicines, especially in the design of new drugs which are active in brain tissue. In particular, the importance of brain-to-blood transport of brain-derived metabolites across the BBB has gained increasing attention as a potential mechanism in the pathogenesis of neurodegenerative disorders such as Parkinson's disease (Bartels, 2011) and AD characterized by the aberrant polymerization and accumulation of specific misfolded proteins, particularly β-amyloid (Aβ), a neuropathological hallmark of AD. P-glycoprotein (P-gp or MDR1/ABCB1) is a 170-kDa transmembrane protein widely expressed from the epithelial cells of the intestine, liver, kidney, placenta, uterus, and testis to endothelial cells of the BBB (Gottesman & Pastan, 1993). It belongs to the ABC (ATP-binding cassette) transporter family and serves to pump exogenous substances out of the cells (Suresh et al, 1999). The domain topology of P-gp consist of two homologous halves each consist a transmembrane domain preceding a cytosolic nucleotide binding domain. Each transmembrane domain is composed of six transmembrane α-helix segments involved in efflux as well as in drug binding (Kast et al, 1996). The ABC transport protein P-gp, a major component of the BBB, mediates the efflux of Aβ from the brain as well as a major factor in mediating resistance to brain entry by numerous exogenous chemicals, including therapeutic pharmaceuticals (Bendayan et al, 2002). P-gp plays a role in the etiology of AD through the clearance of Aβ from the brain. Some drugs, such as rifampicin, dexamethasone, caffeine, verapamil, hyperforin, β-estradiol and pentylenetetrazole, were able to improve the efflux of Aβ from the cells via P-gp up-regulation (Abuznait et al, 2011). Meanwhile, some compounds have been shown to reverse the P-gp mediated multidrug resistance (MDR), including verapamil, adriamycin, cyclosporin, and dexverapamil (Kothandan et al, 2011). Harta et al (2010) have shown that up-regulate P-gp in the early stages of AD has the potential to increase Aβ clearance from the brain and reduce Aβ brain accumulation by a transgenic mouse model of AD (human amyloid precursor protein-overexpressing mice). Abuznait et al (2011) have also elucidated the impact of P-gp up-regulation on the clearance of Aβ, which indicated targeting Aβ clearance via P-gp up-regulation effective in slowing or halting the progression of AD and the possibility of P-gp as a potential therapeutic target for AD.
P-gp at the BBB functions as an active efflux pump by extruding a substrate from the brain, which is important for maintaining loco-regional homeostasis in the brain and protection against toxic compounds (Bartels, 2011). P-gp is also discovered in various resistant tumor cells and expressed widely in many normal tissues and plays a very important role in drug ADME-Tox (absorption, distribution, metabolism, excretion, and toxicity). MDR is a matter of growing concern in chemotherapy. Cells which express the multidrug resistance phenotype can over-express efflux transporters after exposure to a single agent. As a result, these cells become resistant to the selective agent and cross-resistant to a broad spectrum of structurally and functionally dissimilar drugs. The drug efflux pump P-gp has been shown to promote MDR in tumors as well as to influence ADME properties of drug candidates (Jabben et al, 2012). P-gp is expressed at the BBB, the blood-cerebrospinal fluid barrier, and the intestinal barrier, thus modulating the absorption and excretion of xenobiotics across these barriers. P-gp and its ligands (substrates and inhibitors) are therefore extensively studied both with respect to reversing MDR in tumors and for modifying ADME-Tox properties of drug candidates, such as CNS active agents (Jabben et al, 2012). P-gp possesses broad substrate specificity and substrates include members of many clinically important therapeutic drug classes, including anti-HIV protease inhibitors, calcium channel blockers used in the treatment of angina, hypertension, antibiotics and cancer chemotherapeutics (Stouch & Gudmundsson, 2002). In this active efflux process, energy originating from ATP hydrolysis is directly consumed. Because of such a wide distribution of P-gp, so if a drug such as quinidine or verapamil inhibits the function of P-gp, it will also inhibit the excretion of digoxin by P-gp leading to increased plasma levels and toxicity due to digoxin. It is believed to be an important protective mechanism against environmental toxins (Martin, 2004). Since the function of P-gp always results in lack of intracellular levels of the drug necessary for effective therapy, the overexpression of P-gp in certain malignant cells is always associated with MDR phenotype (Sharom, 1997). Although recently low resolution structure of P-gp is obtained, its physiological function and mechanisms of MDR modulation are still not very clear (Li et al, 2005). It is well known that a large number of structurally and functionally diverse compounds act as substrates or modulators of P-gp, including calcium and sodium channel blockers, calmodulin antagonists and structural analogues, protein kinase C inhibitors, steroidal and structurally related compounds, indole alkaloids, cyclic peptides and macrolide compounds, flayanoids and miscellaneous compounds (Wang et al, 2003), which mostly share common structural features, such as aromatic ring structures and high lipophilicity. Some of them possess MDR reversing activity. But only a small number of them have entered clinical study and classification of candidate drugs as substrates or inhibitors of the carrier protein is of crucial importance in drug development (Wang et al, 2005).
On the other hand, the prerequisite to cure neurological disorders is that the drug distribution in CNS can reach effectively therapeutic concentrations (Chen et al, 2009). Usually, the high BBB penetration is needed for drugs that activate in brain. The molecule negotiating the BBB must go through cellular membranes comprising of a lipid bilayer. Until now, it is widely accepted that interaction of compounds with P-gp is a complex process and at this time the details of its mechanism of action are still the subject on hot debate. Although the experimental analysis of drug permeability is essential but the procedure of experiment is time consuming and complicated, a theoretical model of drug permeability is effective to give predictions. Membrane-interaction (MI)-QSAR (quantitative structure-activity relationship) method is a structure-based design methodology combined with classic intramolecular QSAR analysis to model chemically and structurally diverse compounds interacting with cellular membranes. Our modified MI-QSAR method that combines QSAR with solute-membrane-water complex simulating the BBB environment is more close to the body condition than MI-QSAR and possesses higher ability to predict organic compounds across BBB (Chen & Yang, 2006). Before we construct any QSAR models, several things should be consider seriously first. There are several critical assumptions that can influence validity and correctness of any QSAR study as follows: the same mechanism of action of all studied analogs; a comparable manner of their binding to the receptor; correlation of binding to the interaction energies; correlation of measured biological activities to the binding affinities (Kubinyi, 1995). All the accuracy answer and research based on the questions above may guarantee that proper and reliable relationships are obtained. However, in case of MDR modulators different mechanisms and different binding sites may be involved. Several screening assays can help in the identification of substrates and inhibitors although they have both advantages and drawbacks, such as cytotoxity assays (Wiese & Pajeva, 2001), inhibition of efflux assays (Stouch & Gudrmundsson, 2001), P-gp-ATPase activation assays, and drug transport assays (Taub et al, 2005).
The goal of a QSAR study is to find a means of predicting the activity of a new compound. If possible, a desirable goal is the understanding of the biology and chemistry that give rise to that activity and the consequential possibility of reengineering the compound to remove or enhance that activity. One successful example is the transformation of nalidixic acid with the help of QSAR into an important family of drug: the quinolone carboxylates, such as norfloxacin, fleroxacin, ciprofloxacin, and levofloxacin (Alka, 2003). Since the method was established in the 1960s, QSAR equations have been used to describe the biological activities of thousands of different drugs and drug candidates (Kuo et al, 2004). The method definitely provides a more accurate way to synthesize or filtrate the new chemical compounds. At last, the final destination is to degrade the cost of research and manufacture. To date, so many methods have been used in QSAR study and some of them have got successful results. There are general methods used in the literatures these years, such as multiple linear regression (MLR) method, partial least square regression (PLSR) (Li et al, 2005), MI-QSAR analysis (Chen & Yang, 2006), and three-dimension (3D) QSAR (Cramer et al, 1988), and artificial neural network (ANN) (Chen et al, 2006). In order to get more accurate results and QSAR models, we have used two different analyses: MLR and PLSR. Moreover, we focus on constructing theoretical models of the interaction between organic compounds and P-gp as well as the predictive models of blood-brain barrier partitioning of organic compounds on the basis of QSAR analysis and MI-QSAR analysis.
2. Materials and methods
2.1. P-glycoprotein ligands
Similarly, another 21 propafenone analogs were selected from the literature of Diethart Schmid et al (1999) and used in QSAR analysis (table 2). In this test Ka of P-gp ATPase in the adriamycin-resistant subline CCRF ADR5000 was used as biological activity for the whole dataset (Schmid et al, 1999). The assays were performed based on the colorimetric determination of inorganic phosphate released by the hydrolysis of ATP. Table 2 shows all the structures and the experimental biological activity value.
Finally, all two-dimensional structures of these compounds mentioned above were constructed using the chemical drawing software ChemDraw 8.0 and prepared for the next calculation.
The energy parameters root in the results of molecular mechanism and molecular dynamics. The total energy of a system expressed as follows (Iyer et al 2002):
Here, the valence interactions includes bond stretching (bond), valence angle bending (angle), dihedral angle torsion (torsion), and inversion, also called out-of-plane interactions (oop) terms, which are part of nearly all forcefields for covalent systems. A Urey-Bradley term (UB) may be used to account for interactions between atom pairs involved in 1-3 configurations (i.e., atoms bound to a common atom):
With the aid of Chemoffice Chem3D Ultra 8.0 and Hyperchem 7.5, we calculated the following descriptors by the procedure in detail below: (1) Draw the structures in ChemDraw 8.0; (2) Change structures to 3D by Chem3D; (3) Considering our chosen compounds, minimize the energy of the molecule based on molecular mechanism MM2 Force Field (Because under the MM2 force field, the time required for performing computations increases as N2, where N is the number of atoms.). We have chosen the job type as minimize energy to minimum RMS (root mean square) Gradient of 0.100 (the default value of 0.100 is a reasonable compromise between accuracy and speed). (4) Under the menu of Analyze-compute properties, select the properties to calculate and get every descriptor value of each compound.
Similarly, a training set of 18 structurally diverse propafenone analogs (table 2) are measured is used to construct QSAR models. The QSAR models are optimized using MLR fitting and stepwise method (Eq.7-Eq.11). Another QSAR modeling was constructed by PLSR (Eg. 12). A test set of five compounds is evaluated using the QSAR models as part of a validation process.
2.2. Blood-brain-barrier
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B1 |
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-0.04 | B20 |
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0.85 |
B2 |
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-2.00 | B21 |
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0.03 |
B3 |
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-1.30 | B22 |
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0.37 |
B4 |
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-1.06 | B23 |
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-0.15 |
B5 |
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0.11 | B24 |
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-0.17 |
B6 |
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0.49 | B25 |
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0.97 |
B7 |
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-1.17 | B26 |
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1.04 |
B8 |
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-0.18 | B27 |
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0.08 |
B9 |
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-1.15 | B28 |
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0.40 |
B10 |
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-1.57 | B29 |
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0.24 |
B11 |
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-0.46 | B30 |
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-0.16 |
B12 |
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-0.24 | B31 |
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0.13 |
B13 |
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-0.02 | B32 |
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0.35 |
B14 |
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0.44 | B33 |
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0.93 |
B15 |
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0.14 | B34 |
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-0.16 |
B16 |
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0.22 | B35 |
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0.27 |
B17 |
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-0.06 | B36 |
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0.37 |
B18 |
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-1.40 | B37 |
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0.34 |
B19 |
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0.25 | |||
T1 |
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-0.08 | T5 |
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0.81 |
T2 |
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1.01 | T6 |
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0.04 |
T3 |
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0.90 | T7 |
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0.76 |
T4 |
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0.00 | T8 |
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-0.15 |
3. Results
3.1. QSAR analysis based on MDR ratio in P388/VDR-20 and KB-A1 in vitro
Take MDR ratio in vitro in KB-A1/ADR cell lines as dependent variable and molecule descriptors as independent variable. A training set of 26 structurally diverse compounds (Table 4) was used to construct QSAR models. The QSAR models were optimized using MLR fitting and stepwise method by the SPSS software (Eq.1-Eq.5). A test set of 5 compounds (compound A27-A31) was evaluated using the models as part of a validation process (figure 2 upper, Table 5).
Meanwhile, take MDR ratio in vitro in P388/VDR cell lines as dependent variable and molecule descriptors as independent variable. With the aid of Virtual Computational Chemistry Laboratory software (http://vcclab.org) (Wang et al, 2005), construct QSAR modeling by PLSR (Eg.6, figure 2 down). Table 6 shows the calculated descriptors mentioned above and the result of predicted value was in Table 5.
A1 | 1.20 | 37.03 | 2662570 | 3.33 | -3.56 | A14 | 1.22 | 39.02 | 3358755 | 1.48 | -19.64 |
A2 | 1.18 | 35.03 | 2440928 | 2.59 | -13.71 | A15 | 1.22 | 39.02 | 3358755 | 1.48 | -19.71 |
A3 | 1.22 | 40.02 | 3649082 | 1.14 | -16.23 | A16 | 1.20 | 37.03 | 2662570 | 2.13 | -15.99 |
A4 | 1.14 | 32.03 | 1669953 | 2.21 | -13.54 | A17 | 1.202 | 37.03 | 2662570 | 2.13 | -16.23 |
A5 | 1.22 | 39.02 | 3358755 | 1.33 | -19.71 | A18 | 1.202 | 37.03 | 2662570 | 2.13 | -15.95 |
A6 | 1.20 | 37.03 | 2662570 | 2.13 | -16.22 | A19 | 1.18 | 37.03 | 3091919 | 1.61 | -15.9 |
A7 | 1.22 | 40.02 | 3491392 | 0.76 | -17.67 | A20 | 1.23 | 41.02 | 4008723 | 0.76 | -17.36 |
A8 | 1.20 | 37.03 | 2662570 | 2.28 | -16.3 | A21 | 1.14 | 32.03 | 1651352 | 1.9 | -13.79 |
A9 | 1.24 | 42.02 | 4491514 | 1.29 | -16.34 | A22 | 1.22 | 39.02 | 3324212 | 1.33 | -20.06 |
A10 | 1.24 | 41.02 | 4055919 | 0.99 | -19.77 | A23 | 1.20 | 37.03 | 2634052 | 2.13 | -15.77 |
A11 | 1.18 | 36.03 | 2271976 | 1.41 | -17.73 | A24 | 1.19 | 36.03 | 2246188 | 2.13 | -16.15 |
A12 | 1.19 | 36.03 | 2271976 | 2.13 | -16.17 | A25 | 1.15 | 35.03 | 2244801 | 1.71 | -14.88 |
A13 | 1.15 | 33.03 | 1900460 | 2.28 | -13.57 | A26 | 1.15 | 35.03 | 2271261 | 1.71 | -15.03 |
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A27 | 1.19 | 37.03 | 2662570 | 1.41 | -18.09 | A30 | 1.25 | 41.02 | 3977672 | 2.98 | -13.52 |
A28 | 1.22 | 40.02 | 3491392 | 0.76 | -17.61 | A31 | 1.20 | 37.03 | 2634052 | 2.13 | -15.95 |
A29 | 1.21 | 37.03 | 2662570 | 2.75 | -15.55 |
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A1 | 171 | 114.32 | 215.61 | 200.33 | 123.15 | 180.87 | A14 | 147 | 151.94 | 151.04 | 171.02 | 173.75 | 144.79 |
A2 | 278 | 80.79 | 200.54 | 305.22 | 260.52 | 228.39 | A15 | 152 | 150.27 | 140.09 | 157.75 | 159.16 | 130.87 |
A3 | 238 | 161.08 | 71.37 | 78.37 | 79.12 | 92.55 | A16 | 209 | 115.64 | 233.15 | 217.87 | 209.32 | 197.83 |
A4 | 236 | 44.84 | 113.11 | 178.94 | 196.99 | 213.61 | A17 | 171 | 115.64 | 233.15 | 217.87 | 209.32 | 193.94 |
A5 | 160 | 150.27 | 140.09 | 157.75 | 168.14 | 148.66 | A18 | 156 | 116.97 | 252.09 | 236.91 | 229.26 | 219.10 |
A6 | 208 | 113.02 | 199.36 | 184.18 | 174.42 | 159.21 | A19 | 49 | 81.98 | 22.31 | 33.79 | 29.47 | 25.56 |
A7 | 102 | 163.01 | 77.39 | 67.24 | 80.67 | 105.63 | A20 | 214 | 198.44 | 93.91 | 119.73 | 132.46 | 165.76 |
A8 | 120 | 114.32 | 215.61 | 200.33 | 180.88 | 153.75 | A21 | 113 | 42.69 | 80.90 | 121.41 | 145.60 | 174.56 |
A9 | 75 | 237.62 | 101.82 | 179.28 | 149.94 | 146.81 | A22 | 200 | 150.27 | 140.09 | 149.67 | 160.44 | 139.02 |
A10 | 136 | 222.49 | 204.96 | 297.19 | 322.30 | 315.82 | A23 | 189 | 113.02 | 199.36 | 176.36 | 167.80 | 160.14 |
A11 | 44 | 79.86 | 58.80 | 41.66 | 49.61 | 53.08 | A24 | 142 | 92.42 | 159.30 | 116.68 | 117.52 | 112.54 |
A12 | 83 | 92.42 | 159.30 | 121.35 | 121.70 | 115.60 | A25 | 6 | 52.12 | 10.08 | 9.16 | 8.45 | 8.02 |
A13 | 272 | 53.80 | 124.41 | 185.32 | 190.50 | 197.66 | A26 | 9 | 52.12 | 10.08 | 9.53 | 8.76 | 8.16 |
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A27 | 406 | 99.21 | 81.97 | 70.98 | 80.61 | 81.67 | A30 | 370 | 243.10 | 375.08 | 504.47 | 282.78 | 192.47 |
A28 | 68 | 163.01 | 77.39 | 67.24 | 80.67 | 106.16 | A31 | 210 | 114.32 | 215.61 | 191.82 | 183.83 | 174.21 |
A29 | 723 | 125.69 | 411.51 | 400.76 | 323.36 | 248.59 |
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A1 | 50 | 43.66 | 3.33 | 15.85 | 32.21 | 37.03 | 5476 | A18 | 129 | 62.87 | 2.13 | 15.90 | 27.08 | 37.03 | 5476 |
A2 | 78 | 40.71 | 2.59 | 15.10 | 21.84 | 35.08 | 4872 | A19 | 36 | 29.48 | 1.61 | 15.13 | 21.63 | 37.03 | 5585 |
A3 | 75 | 53.15 | 1.14 | 16.63 | 24.83 | 40.02 | 6522 | A20 | 70 | 73.87 | 0.76 | 17.12 | 25.52 | 41.02 | 6855 |
A4 | 53 | 55.39 | 2.21 | 13.91 | 20.16 | 32.03 | 3916 | A21 | 35 | 54.41 | 1.9 | 13.82 | 20.17 | 32.03 | 3874 |
A6 | 93 | 86.84 | 2.13 | 15.83 | 32.75 | 37.03 | 5476 | A24 | 24 | 24.57 | 2.13 | 15.39 | 23.42 | 36.03 | 4855 |
A8 | 30 | 47.64 | 2.28 | 15.85 | 25.21 | 37.03 | 5476 | A25 | 13 | 11.32 | 1.71 | 14.21 | 22.20 | 35.03 | 4487 |
A9 | 57 | 79.51 | 1.29 | 17.56 | 26.03 | 42.02 | 7353 | A26 | 24 | 11.44 | 1.71 | 14.21 | 20.92 | 35.03 | 4538 |
A10 | 108 | 138.69 | 0.99 | 17.40 | 29.44 | 41.02 | 6935 | A27 | 84 | 58.01 | 1.41 | 15.54 | 26.05 | 37.03 | 5476 |
A11 | 37 | 30.21 | 1.41 | 15.08 | 24.04 | 36.03 | 4909 | A28 | 57 | 35.88 | 0.76 | 16.66 | 23.78 | 40.02 | 6244 |
A12 | 15 | 27.61 | 2.13 | 15.39 | 23.512 | 36.03 | 4909 | A29 | 108 | 49.03 | 2.75 | 16.06 | 25.95 | 37.03 | 5476 |
A13 | 78 | 87.23 | 2.28 | 14.27 | 29.12 | 33.03 | 4216 | A30 | 27 | 35.79 | 2.98 | 17.61 | 26.49 | 41.02 | 6804 |
A14 | 56 | 96.24 | 1.48 | 16.50 | 28.19 | 39.02 | 6288 | A32 | 59 | 30.18 | 1.83 | 15.13 | 22.08 | 37.03 | 5642 |
A15 | 75 | 89.20 | 1.48 | 16.47 | 27.54 | 39.02 | 6288 | A33 | 71 | 73.84 | 0.86 | 15.79 | 27.62 | 38.03 | 5822 |
A16 | 51 | 54.90 | 2.13 | 15.88 | 25.61 | 37.03 | 5476 | A34 | 13 | 31.95 | 2.58 | 15.64 | 25.36 | 37.03 | 5476 |
A17 | 70 | 54.43 | 2.13 | 15.88 | 25.49 | 37.03 | 5476 | A35 | 3 | 12.22 | 1.71 | 14.21 | 20.40 | 35.03 | 4589 |
3.2. QSAR analysis based on Ka of ATPase in CCRF ADR5000 cell lines
Similarly, take Ka of ATPase in CCRF ADR5000 cell lines as dependent variable and molecule descriptors as independent variable. We construct QSAR models using two methods, MLD method (Eq.7-Eq.11) and PLSR method (Eg.12) (see figure 3).
A training set of 16 structurally diverse compounds was used to construct QSAR models. All the molecular descriptors were calculated as Table 7. The QSAR models were optimized using MLR fitting and stepwise method. A test set of 2 compounds was evaluated using the models as part of a validation process. Table 8 displays the comparison of the experiment and prediction value.
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A36 | 3.39 | 21.04 | 9.254 | -9.14 | 1366 | 312.41 | A45 | 4.3 | 26.04 | 11.42 | -9.17 | 2345 | 383.53 |
A37 | 3.62 | 24.04 | 10.55 | -9.20 | 1949 | 355.48 | A46 | 4.93 | 32.03 | 13.27 | -8.24 | 4689 | 462.57 |
A38 | 3.67 | 25.04 | 10.84 | -9.16 | 2172 | 367.49 | A47 | 5.2 | 32.03 | 13.38 | -8.19 | 4329 | 464.58 |
A39 | 1.42 | 18.05 | 7.86 | -9.12 | 920 | 277.37 | A48 | 4.25 | 26.04 | 11.45 | -9.24 | 2607 | 383.53 |
A40 | 4.93 | 32.03 | 13.27 | -8.16 | 4329 | 462.57 | A49 | 4.52 | 26.04 | 11.59 | -8.94 | 2367 | 385.55 |
A41 | 2.67 | 25.04 | 10.29 | -8.15 | 2244 | 372.44 | A50 | 4.88 | 27.03 | 12.06 | -8.94 | 2550 | 399.58 |
A42 | 0.94 | 19.05 | 8.01 | -9.15 | 1050 | 293.37 | A51 | 2.38 | 26.04 | 10.99 | -9.09 | 2400 | 383.49 |
A43 | 2.54 | 25.04 | 10.52 | -9.20 | 2172 | 369.46 | A52 | 3.94 | 25.04 | 10.95 | -9.05 | 2172 | 369.51 |
A44 | 3.98 | 32.03 | 13.50 | -9.16 | 4227 | 459.59 | A53 | 4.93 | 32.03 | 13.27 | -8.19 | 4509 | 462.57 |
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Eg.7 | Eg.8 | Eg.9 | Eg.10 | Eg.11 | Eg.12 | Eg.7 | Eg.8 | Eg.9 | Eg.10 | Eg.11 | Eg.12 | ||||
A36 | 3.34 | 6.07 | 12.75 | 9.37 | 6.43 | 6.14 | 13.57 | A45 | 1.53 | 2.20 | 3.02 | 3.32 | 2.69 | 2.08 | 3.50 |
A37 | 5.30 | 4.70 | 6.62 | 7.10 | 6.19 | 5.60 | 7.33 | A46 | 1.47 | 1.09 | 0.73 | 0.52 | 0.48 | 0.81 | 1.02 |
A38 | 2.59 | 4.44 | 5.41 | 5.36 | 3.98 | 3.06 | 6.24 | A47 | 0.55 | 0.81 | 0.61 | 0.46 | 0.50 | 0.53 | 0.84 |
A39 | 122 | 54.54 | 76.92 | 73.09 | 90.64 | 160.46 | 70.37 | A48 | 7.64 | 2.33 | 3.13 | 3.83 | 3.33 | 4.22 | 3.60 |
A40 | 0.36 | 1.09 | 0.73 | 0.52 | 0.53 | 0.51 | 1.02 | A49 | 12.20 | 1.72 | 2.62 | 3.39 | 4.98 | 5.00 | 2.99 |
A41 | 6.13 | 13.54 | 10.43 | 7.17 | 11.79 | 7.23 | 11.56 | A50 | 2.26 | 1.15 | 1.75 | 2.37 | 3.50 | 3.28 | 2.04 |
A42 | 120.00 | 93.12 | 89.09 | 81.21 | 80.47 | 99.37 | 80.44 | A51 | 10.50 | 18.71 | 10.66 | 14.57 | 16.6 | 13.20 | 12.02 |
A43 | 18.50 | 15.65 | 11.36 | 11.73 | 8.26 | 5.56 | 12.59 | A52 | 12.80 | 3.29 | 4.53 | 4.74 | 4.57 | 3.91 | 5.15 |
A44 | 1.01 | 3.15 | 1.36 | 2.10 | 1.66 | 2.13 | 1.88 | A53 | 4.15 | 1.09 | 0.73 | 0.52 | 0.51 | 0.65 | 1.02 |
3.3. QSAR analysis based on blood-brain barrier partitioning of organic compounds
37 organic compounds of training set and 8 compounds of test set are built and minimized, dissolved in liquid, and are optimized by Monte Carlo method and molecular mechanism, finally the dominant conformation of these compounds are obtained. Molecular modeling of a small molecule complex with the membrane-water model reveals that the energy of an organic compound inserted at the middle position in the DMPC model with a layer of water is lower than that of the other two positions. MI-QSAR analysis has been used to develop predictive models of some organic compounds through BBB, in part, simulating the interaction of an organic compound with the phospholipide-rich regions of cellular membranes surrounding by a layer of water. Molecular descriptors of compounds in a training set and a test set are listed in Table 9. Six QSAR equations were constructed based on Table 9 and were listed as follows.
Here, n means the number of compounds in a training set,
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B1 | 78.90 | 1.20 | 12378 | -1.35503 | -298.2972 | -1713.1146 | 42.46 | 11.30 |
B2 | 94.00 | 1.99 | 1101758 | -0.15595 | -406.0803 | -1789.8084 | -65.32 | -65.39 |
B3 | 73.00 | 3.80 | 1738650 | -1.48472 | -256.3021 | -1703.1425 | 84.46 | 21.27 |
B4 | 87.00 | 1.63 | 1346396 | -1.39112 | -302.7543 | -1841.5635 | 38.00 | -117.15 |
B5 | 39.00 | 1.02 | 41807 | 0.58131 | -226.3773 | -1734.7452 | 114.38 | -10.33 |
B6 | 26.80 | 3.23 | 305770 | -0.09264 | -228.2923 | -1679.4604 | 112.47 | 44.96 |
B7 | 88.80 | 1.01 | 58510 | 0.71038 | -279.0781 | -1671.3414 | 61.68 | 53.07 |
B8 | 76.60 | 2.80 | 62216 | -0.38334 | -309.2981 | -1654.6730 | 31.46 | 69.74 |
B9 | 104.40 | 1.77 | 83798 | -0.35599 | -313.4237 | -1639.9898 | 27.34 | 84.43 |
B10 | 108.80 | 2.00 | 193593 | -0.52172 | -548.5593 | -1640.9214 | -207.80 | 83.49 |
B11 | 47.90 | 2.51 | 352512 | -0.09496 | -312.1226 | -1656.7465 | 28.64 | 67.67 |
B12 | 45.20 | 4.27 | 779210 | 0.00479 | -163.8011 | -1716.3101 | 176.96 | 8.11 |
B13 | 38.50 | 2.61 | 158640 | -0.09491 | -170.3338 | -1716.7159 | 170.43 | 7.70 |
B14 | 40.00 | 4.28 | 431722 | -1.30506 | -247.0951 | -1748.0241 | 93.66 | -23.61 |
B15 | 39.20 | 5.88 | 766256 | 0.09911 | -289.2825 | -1735.4004 | 51.48 | -10.98 |
B16 | 54.90 | 5.14 | 766256 | -0.14215 | -181.0636 | -1743.6068 | 159.70 | -19.19 |
B17 | 18.80 | 0.62 | 20863 | 0.18071 | -331.7044 | -1695.6999 | 9.05 | 28.72 |
B18 | 46.70 | 0.27 | 20264 | -1.36843 | -209.4697 | -1644.6752 | 131.29 | 79.74 |
B19 | 44.10 | 2.80 | 190375 | -2.97778 | -311.9182 | -1713.8942 | 28.84 | 10.52 |
B20 | 5.40 | 4.85 | 210631 | -0.06079 | -235.7250 | -1704.3399 | 105.03 | 20.08 |
B21 | 0.00 | -0.47 | 4 | 0.00000 | -407.3194 | -1729.3793 | -66.56 | -4.96 |
B22 | 0.00 | 2.14 | 972 | -0.00009 | -239.8807 | -1675.1827 | 100.88 | 49.23 |
B23 | 23.40 | 0.07 | 213 | 0.00000 | -160.1278 | -1672.3898 | 180.63 | 52.03 |
B24 | 22.60 | 0.69 | 712 | 0.00000 | -319.0674 | -1742.6968 | 21.69 | -18.28 |
B25 | 0.00 | 3.74 | 1899 | 0.00067 | -282.3721 | -1751.6193 | 58.39 | -27.20 |
B26 | 0.00 | 3.61 | 1661 | 0.00000 | -285.7132 | -1731.9518 | 55.05 | -7.54 |
B27 | 0.00 | 1.43 | 1661 | -0.00008 | -238.7249 | -1731.3090 | 102.03 | -6.89 |
B28 | 0.00 | 2.48 | 633 | 0.00003 | -291.5583 | -1725.7370 | 49.20 | -1.32 |
B29 | 11.60 | 2.46 | 21380 | -0.00005 | -418.0323 | -1682.7138 | -77.27 | 41.70 |
B30 | 24.40 | -0.24 | 47 | 0.00000 | -329.3150 | -1704.6187 | 11.44 | 19.80 |
B31 | 10.70 | 1.27 | 7864 | -0.00002 | -253.3453 | -1747.7044 | 87.41 | -23.29 |
B32 | 0.00 | 2.37 | 7322 | -0.00003 | -268.8335 | -1714.2486 | 71.93 | 10.17 |
B33 | 0.00 | 3.31 | 931 | 0.02567 | -353.8395 | -1739.7672 | -13.08 | -15.35 |
B34 | 24.40 | -0.24 | 47 | 0.00000 | -187.4520 | -1720.5500 | 153.31 | 3.87 |
B35 | 0.00 | 1.93 | 7322 | -0.00003 | -177.4875 | -1728.8621 | 163.27 | -4.45 |
B36 | 0.00 | 2.64 | 2050 | -0.02344 | -220.3940 | -1681.1548 | 120.36 | 43.26 |
B37 | 0.00 | 2.63 | 712 | -0.00002 | -231.5752 | -1722.2582 | 109.18 | 2.16 |
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T1 | 22.70 | 0.321 | 712 | 0.00000 | -274.7201 | -1713.7409 | 66.04 | 10.68 |
T2 | 0.00 | 3.738 | 1838 | 0.00000 | -225.6308 | -1716.6234 | 115.13 | 7.79 |
T3 | 0.00 | 4.267 | 4150 | 0.00000 | -331.3754 | -1700.6397 | 9.38 | 23.78 |
T4 | 11.30 | 0.870 | 791 | 0.00000 | -181.5954 | -1700.8447 | 159.16 | 23.57 |
T5 | 0.00 | 4.397 | 4650 | 0.00000 | -404.2903 | -1741.2420 | -63.53 | -16.83 |
T6 | 0.00 | 1.103 | 0 | 0.00000 | -282.9386 | -1746.1889 | 57.82 | -21.77 |
T7 | 0.00 | 3.339 | 791 | 0.00063 | -271.9174 | -1681.9440 | 68.84 | 42.47 |
T8 | 22.70 | -0.208 | 213 | 0.00000 | -364.8884 | -1695.3605 | -24.13 | 29.06 |
With the increase of the variable from one to six, the relativity of QSAR equation is also improved, and the predictive ability of the model is enhanced. Eq.18 is most significant, which means that the capability of an organic compound through BBB depends upon PSA, ClogP, BI, Estretch, ΔEtotal, and ΔEtorsion. Moreover, the potential of an organic compound through BBB is directly proportional to ClogP and ΔEtotal, but inversely proportional to PSA, BI, Estretch, and ΔEtorsion. The observed and predicted log BB values of the training set compounds are listed in Table 10. Figure 4 shows the comparison of the experimental log BB values for all the molecules of the training set with the corresponding predicted log BB as predicted by Eg.17 and -18 MI-QSAR models. Compound B18 in the training set is predicted to have a much higher log BB than observed, and this molecule has also been identified as an outlier in other studies (Iyer et al, 2002). Protonation of the molecule could account for its low log BB value.
A test set of eight solute compounds was constructed as one way to attempt to validate the QSAR models given by six equations mentioned. The test set compounds were selected so as to span almost the entire range in BBB partitioning. The observed and predicted log BB values for this test set are given in Table 10 and plotted in Figure 4 (right). It seems to suggest that Eg.17and -18 QSAR models could predict log BB for other compounds in drug design.
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B1 | -0.04 | -0.81 | -0.95 | -0.71 | -0.52 | -0.33 | -0.20 | B20 | 0.85 | 0.46 | 0.77 | 0.87 | 0.85 | 0.99 | 1.01 |
B2 | -2.00 | -1.07 | -1.11 | -1.44 | -1.56 | -1.57 | -1.39 | B21 | 0.03 | 0.55 | 0.17 | -0.05 | -0.03 | -0.12 | -0.10 |
B3 | -1.30 | -0.71 | -0.51 | -1.20 | -1.11 | -0.98 | -1.17 | B22 | 0.37 | 0.55 | 0.51 | 0.50 | 0.50 | 0.64 | 0.57 |
B4 | -1.06 | -0.95 | -1.04 | -1.58 | -1.49 | -1.37 | -1.13 | B23 | -0.15 | 0.15 | -0.16 | -0.23 | -0.24 | 0.04 | -0.03 |
B5 | 0.11 | -0.12 | -0.30 | -0.26 | -0.40 | -0.19 | -0.06 | B24 | -0.17 | 0.16 | -0.06 | -0.09 | -0.10 | -0.04 | 0.08 |
B6 | 0.49 | 0.09 | 0.20 | 0.19 | 0.16 | 0.34 | 0.28 | B25 | 0.97 | 0.55 | 0.72 | 0.84 | 0.83 | 0.91 | 1.07 |
B7 | -1.17 | -0.98 | -1.15 | -0.91 | -1.11 | -0.90 | -0.86 | B26 | 1.04 | 0.55 | 0.70 | 0.81 | 0.80 | 0.88 | 0.98 |
B8 | -0.18 | -0.77 | -0.71 | -0.38 | -0.38 | -0.22 | -0.22 | B27 | 0.08 | 0.55 | 0.42 | 0.35 | 0.35 | 0.49 | 0.56 |
B9 | -1.15 | -1.25 | -1.31 | -0.97 | -0.99 | -0.79 | -0.81 | B28 | 0.40 | 0.55 | 0.55 | 0.57 | 0.57 | 0.64 | 0.71 |
B10 | -1.57 | -1.33 | -1.36 | -1.05 | -1.05 | -1.16 | -1.20 | B29 | 0.24 | 0.35 | 0.35 | 0.41 | 0.39 | 0.31 | 0.27 |
B11 | -0.46 | -0.28 | -0.26 | -0.26 | -0.31 | -0.21 | -0.32 | B30 | -0.16 | 0.13 | -0.22 | -0.31 | -0.32 | -0.26 | -0.26 |
B12 | -0.24 | -0.23 | 0.02 | -0.13 | -0.23 | 0.03 | 0.04 | B31 | 0.13 | 0.37 | 0.21 | 0.18 | 0.17 | 0.31 | 0.43 |
B13 | -0.02 | -0.11 | -0.08 | 0.01 | -0.02 | 0.26 | 0.34 | B32 | 0.35 | 0.55 | 0.54 | 0.55 | 0.54 | 0.64 | 0.68 |
B14 | 0.44 | -0.14 | 0.11 | 0.17 | 0.33 | 0.51 | 0.64 | B33 | 0.93 | 0.55 | 0.66 | 0.75 | 0.74 | 0.73 | 0.84 |
B15 | 0.14 | -0.13 | 0.33 | 0.30 | 0.17 | 0.26 | 0.33 | B34 | -0.16 | 0.13 | -0.22 | -0.31 | -0.32 | -0.07 | -0.02 |
B16 | 0.22 | -0.40 | -0.03 | -0.06 | -0.15 | 0.10 | 0.22 | B35 | 0.27 | 0.55 | 0.48 | 0.45 | 0.45 | 0.68 | 0.74 |
B17 | -0.06 | 0.23 | -0.01 | -0.07 | -0.11 | -0.07 | -0.09 | B36 | 0.37 | 0.55 | 0.57 | 0.61 | 0.61 | 0.77 | 0.72 |
B18 | -1.40 | -0.26 | -0.53 | -0.50 | -0.28 | -0.02 | -0.14 | B37 | 0.34 | 0.55 | 0.57 | 0.60 | 0.60 | 0.75 | 0.81 |
B19 | 0.25 | -0.21 | -0.15 | -0.05 | 0.45 | 0.59 | 0.62 | ||||||||
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T1 | -0.08 | 0.16 | -0.11 | -0.17 | -0.18 | -0.06 | -0.02 | T5 | 0.81 | 0.55 | 0.81 | 0.97 | 0.96 | 0.88 | 1.02 |
T2 | 1.01 | 0.55 | 0.72 | 0.84 | 0.83 | 0.99 | 1.05 | T6 | 0.04 | 0.55 | 0.37 | 0.28 | 0.29 | 0.37 | 0.47 |
T3 | 0.90 | 0.55 | 0.79 | 0.95 | 0.93 | 0.95 | 0.98 | T7 | 0.76 | 0.55 | 0.67 | 0.75 | 0.75 | 0.84 | 0.81 |
T4 | 0.00 | 0.36 | 0.15 | 0.09 | 0.09 | 0.32 | 0.32 | T8 | -0.15 | 0.16 | -0.18 | -0.28 | -0.29 | -0.28 | -0.31 |
4. Discussion
We have built some predictive models of MDR, Ka and BBB partitioning of organic compounds by simulating the interaction of modulators or drugs interact with P-gp and/or of an organic compound with the phospholipide-rich regions of cellular membranes. As we know in the introduction part, modulators or drugs interact with P-gp and thus reduce the efflux of the cytotoxic compounds will increase the apparent toxicity of the cytotoxic compounds. It is very important to keep in mind that it is based on a general assessment of cytotoxicity and thus may account for more than one acting mechanism in the resistant cells used. So there are many uncertainty factors in the MDR ratio assay method and it is also convinced by our linear regression models. Our research results using two different statistic methods, MLR and PLSR, have revealed that the QSAR equation was also improved and the predictive ability of the models was enhanced with the increase of the variable. Eg.5 is built on KB-A1 cell line with a cytotoxic compound of 2.5μM ADR while Eg.6 is based on P388/VDR-20 cell line with 1.5μM VCR. Here, most of the models gave satisfactory cross-validated Q2 above 0.500, conventional R above 0.800 and less SE values indicating their proper predictive ability. Significant differences between values were examined using two-tailed paired T test provided by SPSS. All the results were considered not significant if P<0.05. Eg.5 model is the most significant and indicated that the capability of P-gp modulators interacted with P-gp depends upon MR, BI, Ehyd, ShA, and LogP. The former three display positive contributions to the MDR activity of P-gp, suggesting that the MDR activity increase accordingly with MR increase. The latter two displays negative contribution to the MDR activity of P-gp.
On the other hand, we have built the predicted models for Ka of ATPase of some compounds using the same statistic methods in order to get a more accurate model. Both models, Eg.11 by MLR and Eg.12 by PLSR, point out that LogP and EHOMO are both important parameters with the affinity for and simulation of the P-gp ATPase. LogP is negative related with the activity of P-gp ATPase, suggesting that the ATPase activity also decrease with the increase of LogP. Figure 3 showed that molecular A39 and A42 have higher Ka value of ATPase and is a departure from other compounds. This may be because they have lower lipophilicity, which is supported by the research results of Diethart Schmid et al (1999). Another significant descriptor EHOMO is positive related with the activity of P-gp ATPase.
In another aspect, BBB partitioning is mainly found to depend upon two parameters, namely PSA and ClogP. With the increase of the variable, the relativity of QSAR equation is also improved, and the predictive ability of the model is enhanced, especially Eq.18 most significant. Moreover, the BBB partitioning measures of the test set compounds were predicted with the same accuracy as the compounds of the training set. The family of these QSAR models reveal that the capability of BBB partitioning of an organic compound focus on six significant features, which are PSA, ClogP, BI, Estretch, ΔEtotal, and ΔEtorsion (Eg. 18). Obviously, two of the six descriptors of the QSAR models have positive regression coefficients and the other four descriptors have negative regression coefficients. The potential of an organic compound through BBB is directly proportional to ClogP and ΔEtotal, but inversely proportional to PSA, BI, Estretch, and ΔEtorsion. Moreover, PSA descriptor is found as a dominant descriptor in these QSAR models, which related to the aqueous solubility of the solute compound along with a direct lipophilicity descriptor (Clark et al, 1999). When the value of PSA of a molecule lessens within the range from 0 to 108.80 Å2, its value of LogBB will increase. This is consistent with the experimental results that the more polarity it possesses, the more difficultly a molecule enters the hydrophobic environment of BBB (Stouch, 1993). BI is the connective index of molecular average total distance, which pertains to the volume parameter. Our research result points it out that with the accretion of its bulk, a molecule more and more difficultly across through BBB by diffusion. However, the value of LogBB of a molecule increases with the increase of ClogP. It means that the hydrophobic molecule can pass through BBB more easily than the hydrophilic molecule does, which is supported by the experimental results (Kaliszan & Markuszewski, 1996). The presence of Estretch descriptor suggests that with the decrease of the stretch-bend energy of a molecule, its value of LogBB increases. Two of the descriptors, found in the log BB QSAR models (Eg.17 and Eq.18), reflect the behavior of the solute in the membrane and the entire membrane-solute complex. Along with the meaning mentioned, ΔEtotal is equivalent to the change in average total potential energy between the triple member complex and the double member complex. Similarly, ΔEtorsion is the difference between the dihedral torsion energy of the triple complex and that of the double complex. Here, the more the change value of ΔEtotal is, the more its value of LogBB increases. This is because small molecule across BBB membrane leads to the change of the structure of the complex. The more changeability of the structure results in greater change of total potential energy, while the accretion of the energy change is the important cause of the increase of the capability of a small molecule through BBB. On the contrary, the less the difference of the torsion energy is, the larger its value of LogBB is. It displays that a small molecule tight combining with the membrane-water complex leads to increase its value of LogBB. And the relationship would suggest that as the solute becomes more flexible within the membrane-water complex, the greater would be its log BB value, which is in agreement with the research results of Iyer M et al (2002).
Several non-MI-QSAR computational models to describe and predict BBB partitioning have been reported that includes other descriptors besides PSA and ClogP (Lombardo et al, 1996; Keseru & Molnar, 2001; Crivori et al, 2000). An alternative, complementary approach to BBB partitioning prediction uses MI-QSAR analysis developed by Iyer M et al (2002). Their research results show that BBB partitioning of an organic compound depend upon PSA, CLogP, and the conformational flexibility of the compounds as well as the strength of their “binding” to the model biologic membrane. The MI-QSAR models indicate that BBB partitioning process can be reliably described for structurally diverse molecules provided interactions of the molecule with the phospholipide-rich regions of cellular membranes are explicitly considered. An extension of these approaches that combines QSAR with solute-membrane-water complex has been developed by us, which is addition of a layer of water on the hydrophilic side of DMPC monolayer membrane in our research. And so, it is more analogous to the truth BBB environment. Our results reveal that the distribution of organic molecules through BBB was not only influenced by the properties of organic solutes, but also related to the property of the solute-membrane-water complex. The former involves the polarity, hydrophobic, size, and conformational freedom degree of organic molecules. The latter deals with the strength of an organic molecule combined with BBB membrane and the structural changeability of a solute-membrane-water complex. Furthermore, the capability of a small molecule across BBB is mainly related to four physicochemical factors, which depend on the relative polarity of a small molecule, the molecular volume, the strength of a small molecule combined with DMPC-water model, and the changeability of the structure of a solute-membrane-water complex. The relative polarity of a small molecule includes two parameters, namely PSA and ClogP. The QSAR model shows that less polarity and more hydrophobic molecules relatively easily pass through BBB and enter brain to cure. The molecular volume involves one parameter, namely BI. The strength of a small molecule combined with DMPC monolayer membrane complex with a layer of water involves one parameter, namely ΔEtorsion. The changeability of the structure of a complex between a small molecule and the membrane-water complex includes one parameter, namely ΔEtotal. The reason for the change of total energy is that small molecule across BBB membrane leads to the change of the structure of the solute-membrane-water complex. The more the changeability of the complex structure is, the more the change value of total energy is, and the more easily a small molecule penetrates BBB.
Cerebral clearance of Aβ is considered to occur via elimination across BBB, as well as proteolytic degradation. Attenuation of its elimination is likely to result in increased cerebral Aβ deposition, which may facilitate progression of AD (Ohtsuki et al, 2010). P-gp detoxifies cells by exporting hundreds of chemically unrelated toxins but has been implicated in MDR in the treatment of cancers. Substrate promiscuity is a hallmark of P-gp activity, thus a structural description of poly-specific drug-binding is important for the rational design of anti-amyloid accumulation drugs, anticancer drugs and MDR inhibitors. The x-ray structure of apo P-gp at 3.8 angstroms reveals an internal cavity of approximately 6000 angstroms cubed with a 30 angstrom separation of the two nucleotide-binding domains. Two additional P-gp structures with cyclic peptide inhibitors demonstrate distinct drug-binding sites in the internal cavity capable of stereoselectivity that is based on hydrophobic and aromatic interactions. Apo and drug-bound P-gp structures have portals open to the cytoplasm and the inner leaflet of the lipid bilayer for drug entry. The inward-facing conformation represents an initial stage of the transport cycle that is competent for drug binding (Aller et al, 2009). Currently, P-gp is identificated as an energy-dependent pump, ATPase activity as an assay in itself is possibly problematical cause it is based upon one assumption that drug-induced ATP hydrolysis reflects transport by the transporter (Stouch & Gudmundsson, 2001). There may be many ways in which this activity could be altered, including direct action on the ATP binding domain. Scientists once observed some compounds such as daunomycin and vinblastine inhibit ATPase activity, but increase in others, suggesting that modulation of ATPase activity is highly dependent on experimental conditions and may not correlate well with the ability of P-gp to transport the drug (Ambudkar et al, 1992; Shapiro & Ling, 1994; Doige et al, 1993). The work of Litman et al was one of the few studies suggesting that affinity between drugs and ATPase activity has no correlation to LogP, but Surface Area (Litman et al, 1997). Because of the less comparability of molecular structures in a training set, our QSAR equation possesses universal significance. However, the precision of QSAR equation is so low that there is still a distance to its application. So a series of organic compounds with similar structures are chosen and consist of a training set, thus the precision of QSAR simulation is largely increased, while the prediction of the analogues through BBB is greatly improved.
5. Conclusion
P-gp is involved in MDR and in neurodegenerative disorders such as Parkinson disease, AD and epilepsy. The xenobiotic efflux pump P-gp limits intracellular drug accumulation by active extrusion of compounds out of cells. P-gp mediates the efflux of Aβ from the brain together with mediating MDR, while P-gp transports neutral or positively-charged hydrophobic substrates with consuming energy from ATP hydrolysis. We have built up theoretical models of the interaction between organic compounds and P-gp and compounds with the affinity for and simulation of the P-gp ATPase. The interaction between compounds and p-gp (P-gp binding or MDR-reversal activity of compounds) is found to depend on LogP, LogMR, and ShA of compounds it transports, which proportional to LogMR while inversely proportional to LogP and ShA (see Eg.1 to Eg.5). Until now we have not convinced that ATPase activity of P-gp is well correlated with the ability of P-gp to transport the drugs. However, our constructed model based on the analogies of purine and propafenone analogs suggests that the enzyme hydrolysis of these compounds largely depends on LogP, MR, ShA, MW and EHOMO, especially positive related to MR but negative to LogP and ShA (see Eg.7 to Eq.11). This shows that the P-gp binding capacity of these compounds shares common characteristics with their ATPase hydrolysis, namely their hydrophobic parameters (such as log P) and steric parameters (eg. MW, ShA, MR, and WI).
Additionally, our constructed MI-QSAR model indicates that the distribution of organic molecules through BBB was not only influenced by organic solutes themselves, but also related to the properties of the solute-membrane water complex, namely interactions of the molecule with the phospholipide-rich regions of cellular membranes. Moreover, our results reveal that the ability of organic molecules permeating across BBB is proportional to LogP but inversely proportional to PSA (see Eg.13 to 18), which is consistent with the research results of Chen and co-worker (2009), namely the increasing PSA decreased LogBB rapidly while LogP positively related to LogBB. It indicates that molecules with higher lipophilic will be partitioned into the lipid bilayer more easily with more chances to penetrate BBB, supported by the research result of Wang et al (2003), namely a large number of structurally and functionally diverse compounds as substrates or modulators of P-gp mostly sharing common structural features, such as aromatic ring structures and high lipophilicity. PSA of CNS active drug should be lower than 90 Å2 (Chen et al, 2009), while the penetration through the BBB is optimal for LogP value in the range 1.5–2.7 (Norinder & Haeberlein, 2002).
Scheme 1.
Flowchart for QSAR analysis of some substrates of P-glycoprotein targeting β-amyloid clearance.
In comparison with the ability of organic molecules permeating across BBB, P-gp binding or MDR-reversal activity of compounds has a negative correlation with LogP. There are two reasons for this phenomenon. Firstly, the compounds with higher liposolubility are more vulnerable to cytochrome P450 metabolism, leading to faster clearance (Waterhouse, 2003). P450 enzymes (CYP450s) catalyze the metabolism of a wide variety of endogenous and exogenous compounds including xenobiotics, drugs, environmental toxins, steroids, and fatty acids. Aminated thioxanthones have recently been reported as P-gp inhibitors as well as its interaction with cytochrome P450 3A4 (CYP3A4), as many substrates of P-glycoprotein and CYP3A4 are common (Palmeira et al, 2012). The second reason is related to the mechanism of P-gp action. According to model proposed by Higgins and Gottesman (1992), after entering into the phospholipid bilayer, compound may interact with P-gp in the inner leaflet of the lipid bilayer. Upon interaction with P-gp, the compound is flipped from the inner leaflet to the outer leaflet of the lipid bilayer. The lipophilic compounds with high LogP enter into cellular membrane easily and intend to retain there, so its opportunity to interact with P-gp increases. The LogP not only offers opportunity to penetrate the lipid bilayer, but also gives favorable contribution to binding with protein, such as P450, P-gp.
In conclusion, the predictive model of BBB partitioning of organic compounds contributes to discovery of some molecules through BBB as potential AD therapeutic drugs. Moreover, the interaction model of P-gp and modulators for treatment of multidrug resistance indicates discovery of some molecules to increase Aβ clearance from the brain and reduce Aβ brain accumulation by regulate BBB P-gp in the early stages of AD. The mechanism suggests new therapeutic strategy in AD.
Acknowledgments
This work was supported by a grant from Basic Scientific Research Expenses of Central University (020814360012), National Key Technology R&D Program (2008BAI51B01) and Specialized Research Fund for the Doctoral Program of Higher Education (20120091110038).
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