Sreenivas Avula1, Xudan Peng1, Xingfen Lang1, Micky Tortorella1,2, Béatrice Josselin3,4, Stéphane Bach3,4, Stephane Bourg5, Pascal Bonnet5, Frédéric Buron5, Sandrine Ruchaud3, Sylvain Routier5, Cleopatra Neagoie1,2. 1. Guangzhou Institute of Biomedicine and Health, Chinese Academy of Science, Guangzhou, China. 2. Centre for Regenerative Medicine and Health, Hong Kong Institute of Science and Innovation, Chinese Academy of Science, Hong Kong SAR, China. 3. Sorbonne Université/CNRS UMR8227, Roscoff cedex, France. 4. Sorbonne Université/CNRS FR2424, Plateforme de criblage KISSf (Kinase Inhibitor Specialized Screening Facility), Roscoff cedex, France. 5. Institut de Chimie Organique et Analytique, Université d'Orléans, UMR CNRS 7311, Orleans, France.
Abstract
A library of substituted indolo[2,3-c]quinolone-6-ones was developed as simplified Lamellarin isosters. Synthesis was achieved from indole after a four-step pathway sequence involving iodination, a Suzuki-Miyaura cross-coupling reaction, and a reduction/lactamization sequence. The inhibitory activity of the 22 novel derivatives was assessed on Haspin kinase. Two of them possessed an IC50 of 1 and 2 nM with selectivity towards a panel of 10 other kinases including the parent kinases DYRK1A and CLK1. The most selective compound exerted additionally a very interesting cell effect on the osteosarcoma U-2 OS cell line.
A library of substituted indolo[2,3-c]quinolone-6-ones was developed as simplified Lamellarin isosters. Synthesis was achieved from indole after a four-step pathway sequence involving iodination, a Suzuki-Miyaura cross-coupling reaction, and a reduction/lactamization sequence. The inhibitory activity of the 22 novel derivatives was assessed on Haspin kinase. Two of them possessed an IC50 of 1 and 2 nM with selectivity towards a panel of 10 other kinases including the parent kinases DYRK1A and CLK1. The most selective compound exerted additionally a very interesting cell effect on the osteosarcoma U-2 OS cell line.
Marine products currently represent an underutilised source of leads for the pharmaceutical industry. Besides their original and complex structures, they often offer new action modes and structural originality. Nevertheless, their low abundance and the presence of few analogues makes it difficult to obtain large libraries, perform full biological characterisation and achieve structure–activity relationship (SAR) exploration. Despite these difficulties, these products remain attractive due to their high valorisation potential, and their complex structures have prompted medicinal chemists to use disruptive strategies to intuitively isolate the pharmacophore elements that trigger biological activity.For these reasons, some marine products and their synthetic analogues have emerged in drug discovery strategies and several of them have been reported for protein kinase inhibition. Among them the most successful example is the polycyclic staurosporine I,. This lead compound has led from extraction, hemisynthesis and organic synthesis efforts to Lestaurtinib II, and simplified Enzastaurin III, two potent drugs targeting VEGF receptors and kinases, which have entered clinical trials against leukaemia and cancer (Figure 1). In this field, the chemical simplification of indolocarbazole scaffolds and caulersin IV have generated strong kinase inhibitors and cytotoxic agents.
Figure 1.
Structures of Staurosporine and its simplified derivatives, which have entered clinical trials as kinase inhibitors, and Caulersin.
Structures of Staurosporine and its simplified derivatives, which have entered clinical trials as kinase inhibitors, and Caulersin.Among these bis-indole series, lamellarins, a group of pyrrole alkaloids, have emerged (Figure 2),. These compounds are a class of marine-derived natural products isolated from molluscs, ascidians and marine sponges. Nearly, 70 natural derivatives have been reported in this family which mainly contains a fused pentacyclic pyrroloisoquinoline lactone ring system. Lamellarins have focussed the attention of medicinal chemists due to their diverse biological effects. Some have demonstrated cytotoxic activities and multidrug resistance (MDR) reversal in a number of cancer cell lines, as well as being confirmed inhibitors of topoisomerase I. Moreover, Lamellarins D (structure V, Figure 2), N and L have proved their ability to inhibit kinases such as GSK3β, DYRK1A and CDK5 in the nanomolar range. Our first approach in this chemical series was based on the simplification of the synthetic model in order to discriminate the two activities, that is, diminish the topoisomerase I inhibition while retaining the kinase inhibition by fine-tuning the chemical structure.
Figure 2.
Lamellarin D, chromenoindoles, and envisioned indoloquinolinone chemical series.
Lamellarin D, chromenoindoles, and envisioned indoloquinolinone chemical series.This objective was reached by replacing the pyrrole moiety with an indole skeleton and designing new chromeno[3,4-b]indoles VI which revealed DYRK1A inhibition. In this structure, the rings of Lamellarin-D noted A, B and C were unchanged (Figure 2). Despite structural modulations, the kinase inhibition remained mainly in the sub-micromolar range except for derivatives 1a and 1b, which exhibited a high selective inhibition of DYRK1A but revealed instability in basic media due to the lactone. We therefore decided to develop a more robust indoloquinolinone series VII with the objective of creating a novel and druggable family of kinase inhibitors, as we envisioned that the presence of lactam combined with the NH of pyrrole would reinforce the hydrogen bond donor acceptor binding mode to the ATP active site.Herein, we present access to the indolo[2,3-c]quinolone-6-one library and the evaluation of the family on a representative panel of kinases involved in CNS, inflammatory diseases and oncology. SAR are depicted and we demonstrate that in addition to retaining DYRK1A inhibition to a large extent, other molecules acting on CLK1 have also been designed. We additionally found that several compounds inhibit the Haspin kinase with an unprecedented selectivity. Molecular docking experiments were conducted to explain these results. Finally, screening on a cancer cell line was carried out and results showed that the compounds induced cellular effects and affect osteosarcoma cell lines in particular.
Chemistry
In order to introduce ring A on the indole, a Suzuki-Miyaura reaction appeared to be the most appropriate. The 3-iodoindole-2-carboxylic ethyl esters 10–13 were therefore prepared after 2 efficient steps. The first one consisted in the quantitative esterification of 2–4 using 10 mol% of sulphuric acid catalyst in ethanol, followed by iodination in presence of KOH to afford the attempted ethyl 3-iodo-1H-indolo-2-carboxylates. Noteworthy, the N-methylation of indole 11 with a slight excess of iodomethane in presence of sodium hydride gave 14 in a near quantitative yield (Scheme 1).
Scheme 2.
Reagents and conditions: (i) PhMgCl 2 M in THF (1.2 equiv.), B(OCH3)3 (1.2 equiv.), 30 min. at -78 °C, then aq. HCl 2 M at -10 °C, 10 min; (ii) PdCl2(dppf) (0.03 equiv.), KOAc (2.0 equiv.), Bis-(pinacolato)diboron (1.5 equiv.), 1,4-dioxane/H2O 10/1, 80 °C, 14 h.
Reagents and conditions: (i) EtOH, conc. H2SO4 10 mol%, reflux, 12 h, 6–9 quant.; (ii) I2 (1.5 equiv.), KOH (4.0 equiv.), DMF, r.t., 4 h; (iii) NaH (1.5 equiv.), CH3I (1.2 equiv.), DMF, 0–20 °C.Next, we focussed on preparing the second partner for the cross coupling reaction, that is, the unavailable boronylated nitrobenzene derivatives (Scheme 2). When the starting 2-halogeno nitrobenzenes do not contain any acidic proton, the use of Grignard reagent is recommended in the literature. The reaction was first carried out with phenyl magnesium chloride (1.2 equiv.) in presence of methylorthoborate as electrophile whereas a final acidic hydrolysis led to the desired 2-nitroaryl boronic acids 15–20 in fair good yields. When 2-halogeno nitrobenzenes bear an acidic proton, the Miyaura borylation reaction can be used with conditions involving PdCl2(dppf) as catalyst and potassium acetate as a base in dioxane. This method furnished pinacol boronic esters 21–24 with modest yields after 14 h of reaction at 80 °C. Due to their sensitivity during the purification step, the boron derivatives were used in the cross coupling reaction as crude materials.Reagents and conditions: (i) PhMgCl 2 M in THF (1.2 equiv.), B(OCH3)3 (1.2 equiv.), 30 min. at -78 °C, then aq. HCl 2 M at -10 °C, 10 min; (ii) PdCl2(dppf) (0.03 equiv.), KOAc (2.0 equiv.), Bis-(pinacolato)diboron (1.5 equiv.), 1,4-dioxane/H2O 10/1, 80 °C, 14 h.Assembly of the two building blocks was next performed using the Suzuki-Miyaura reaction in presence of PdCl2(dppf) and potassium carbonate as base in a refluxing mixture of water and dioxane. These conditions proved fully suitable to achieve all the envisioned cross couplings and the desired derivatives were isolated with yields ranging between 40 and 60% after 12 h of reaction (Table 1). Finally, we thought that the large library of final compounds 45–64 could be obtained by a “one pot” strategy (Table 2). To this end, the nitro derivatives 25–44 were also treated with iron powder in refluxing acetic acid and the in situ formed amine concomitantly formed the lactam ring by annelation with the nearby ethyl ester. An original library of substituted 5,7-dihydro-6H-indolo[2,3-c]quinolin-6-ones 45–65 was obtained with very high yields.
Table 1.
Suzuki-Miyaura reaction using 10–14 and boronylated derivatives 15–24.
Entry
Starting materials
Producta(Formula/number)
Entry
Starting materials
Producta(Formula/number)
1
10 + 15
11
11 + 22
2
10 + 17
12
11 + 23
3
10 + 21
13
11 + 24
4
10 + 22
14
12 + 15
5
11 + 15
15
12 + 17
6
11 + 16
16
13 + 17
7
11 + 17
17
13 + 22
8
11 + 18
18
14 + 22
9
11 + 19
19
14 + 19
10
11 + 21
20
14 + 20
aYields are indicated in the experimental section.
Table 2.
“One pot” reduction of nitro group and lactam formation of derivatives 25–44 leading to final compounds 45–64.
Entry
Starting materials
Producta(Formula/number)
Entry
Starting materials
Producta (Formula/number)
1
25
11
35
2
26
12
36
3
27
13
37
4
28
14
38
5
29
15
39
6
30
16
40
7
31
17
41
8
32
18
42
9
33
19
43
10
34
20
44
aYields are indicated in the experimental section.
Suzuki-Miyaura reaction using 10–14 and boronylated derivatives 15–24.aYields are indicated in the experimental section.“One pot” reduction of nitro group and lactam formation of derivatives 25–44 leading to final compounds 45–64.aYields are indicated in the experimental section.
Kinase assays, SAR
We previously showed that analogues of Lamellarin D, chromeno[3,4-b]indoles, had the ability to inhibit the DYRK1A kinase and it has been shown by different groups that DYRK inhibitors often cross-react with CLKs and with the mitotic kinase Haspin,. We therefore tested the inhibitory activity of the 22 synthesised derivatives on the HsHaspin, MmCLK1 and RnDYRK1A recombinant kinases (Table 3).
Table 3.
Residual activity on a representative panel of 8 protein kinases at 1 μM.
Entry
Compound
% Residual activity at 1 μMa
Haspin
CLK1
DYRK1A
CDK2
CDK5
CDK9
GSK3β
PIM1
1
45
44
67
61
100
100
63
100
86
2
46
6
13
18
80
78
62
86
32
3
47
28
22
33
61
59
20
47
37
4
48
1
4
12
84
87
49
100
63
5
49
2
5
7
73
77
40
39
41
6
50
3
10
5
77
81
51
44
19
7
51
1
5
14
62
70
33
29
36
8
52
2
1
5
58
63
37
22
29
9
53
33
11
36
76
56
56
63
31
10
54
0
11
2
35
59
18
48
9
11
55
0
14
2
38
53
17
20
22
12
56
2
3
7
72
79
37
39
65
13
57
3
2
10
100
100
72
58
37
14
58
59
49
55
62
55
55
51
48
15
59
13
12
21
74
51
41
41
34
18
60
9
31
44
97
100
100
100
100
19
61
0
2
9
57
91
41
71
38
20
62
0
0
2
31
22
6
31
75
21
63
51
19
29
67
68
45
44
42
22
64
39
11
19
100
100
59
81
82
aResidual kinase activity was determined at 1 μM concentration for each compound. The data mean (n = 2) expressed as percentage of maximum activity of the DMSO control.
Residual activity on a representative panel of 8 protein kinases at 1 μM.aResidual kinase activity was determined at 1 μM concentration for each compound. The data mean (n = 2) expressed as percentage of maximum activity of the DMSO control.The selectivity of each derivative was also determined on a representative kinase panel including HsCdk2/Cyc A, HsCdk5/p25, HsCdk9/Cyc E, HsGSK3β and HsPIM1. Interestingly, more than half of the analogues displayed very high activity towards Haspin with a percentage of residual activity at 1 μM close to zero (ranging from 6% for compound 46 to 0% for compounds 61, 54, 55, and 62). Apart from 5 compounds (45, 58, 47, 53, 63, and 64), 17 novel indoloquinolinones showed an interesting selectivity towards Haspin, CLK1 and DYRK1A kinases with moderate activity on CDKs, GSK-3β and PIM1.IC50 for Haspin, CLK1 and DYRK1A were next calculated for 14 compounds showing residual kinase activity ≤25% on Haspin kinase at a concentration of 1 μM (Table 4). It clearly appeared that the lactam moiety favoured DYRK1A inhibition. While the hydroxylated derivatives 1a and 1b displayed good activity on DYRK1A, they are nevertheless the only molecules in their family to present this action whereas the 14 lactams reported in this study exhibited an inhibition below 300 nM. It is possible that due to the electro-donating lactam nitrogen atom (vs. the O of the lactone), the electron density on the carbonyl group is sufficiently modified to strengthen a favourable hydrogen bond in the active site (see molecular modelling studies). Moreover, the fcompounds 48, 49, and 51 (entries 2, 3, 5) appear to be the best DYRK1A inhibitors of the series with more potent IC50 than the lactones 1a and 1b (entry 1).
Table 4.
Measured IC50 values (nM) on Haspin, CLK1 and DYRK1A.
Entry
Compound
Kinase inhibition (IC50)a(IC50 in nM)
Selectivity index
Haspin
CLK1
DYRK1A
CLK1/Haspin
DYRK/Haspin
Ref
1a
ND
ND
74
ND
ND
Ref
1b
ND
ND
67
ND
ND
1
46
7
51
68
7
10
2
48
6
17
19
3
3
3
49
1
13
15
13
15
4
50
7
88
196
13
28
5
51
4
10
41
3
10
6
52
16
78
242
5
15
7
54
4
82
97
21
24
8
55
2
33
130
17
65
9
56
14
213
226
15
16
10
57
34
259
280
8
8
11
59
30
94
73
3
2
12
60
19
122
143
6
8
13
61
5
78
104
16
21
14
62
18
124
131
7
7
aIC50 values were determined on Haspin, CLK1 and DYRK1A when the residual kinase activity was ≤25% on Haspin at a compound concentration of 1 μM in Table 3. They were calculated from a dose-response curve for which each point was measured in duplicate, and reported in nM. Selectivity indexes (SI) were calculated as follows: IC50 DYRK1A or CLK1/IC50 Haspin.
Measured IC50 values (nM) on Haspin, CLK1 and DYRK1A.aIC50 values were determined on Haspin, CLK1 and DYRK1A when the residual kinase activity was ≤25% on Haspin at a compound concentration of 1 μM in Table 3. They were calculated from a dose-response curve for which each point was measured in duplicate, and reported in nM. Selectivity indexes (SI) were calculated as follows: IC50 DYRK1A or CLK1/IC50 Haspin.Effects on cell viability, EC50 on RPE1 and U-2 OS cell linesa.aCells were incubated with increasing doses of each compound (up to 50 µM) for 48 h. Cell viability was determined by MTS assay in triplicate and EC50 (µM) were calculated from the dose-response curves.The concomitant action of DYRK1A inhibitors with CLK1 was confirmed since most of the Haspin inhibitors were also active on DYRK1A and CLK1. The mode of interaction of 49, which is highly active on Haspin and exhibits strong activity on the other two kinases, was studied by molecular docking experiments (see Molecular docking studies section). Considering the two enzymes we can say that compounds 48 and 49 inhibit DYRK1A and CLK1 almost equally in the nanomolar range.As regards to Haspin inhibition, the chemical series of type VII is of great interest. Eight compounds showed an IC50 below 10 nM. Compound 45 (Table 3, entry 1), without any substituent on the aromatic parts, presented no kinase activity. To maximise the inhibition, at least one methoxy OCH3 or hydroxy OH group is required in positions C-2 or C-3 (compounds 46, 48, 50, 51, 54, 55, 61), the amino derivatives or amides being less effective (Table 4, entries 9 and 10).Regarding the indole ring substituents, the absence of a substituent or the presence of an OCH3 or a fluorine in C-10 position did not significantly affect the Haspin inhibition (products 46, 51 and 61, entries 1, 5, 13) when a functional group was also present on the C-2 or C-3 positions of the phenyl ring. Finally, the presence of ether in position C-9 (entry 11 vs. 5) or the methylation of indole (entry 14 vs. 5) made the compounds less effective.The inhibitory activity of compound 49 on Haspin was about 12 times stronger than that of the other two enzymes. At 20 nM this molecule inhibited the 3 enzymes quantitatively. Compound 55 showed an even higher selectivity since the selectivity for CLK1 was identical, but against DYRK1A it rose to a factor of 65. At this stage, we can almost say that at a dose of 20 nM, this molecule shows a dual inhibition of Haspin and CLK1.We further evaluated the selectivity profile of compound 55 on a larger panel of kinases (SelectScreen Whole Panel, Life Technologies). The inhibition profile of 55, evaluated at 1 μM, is depicted on a dendrogram on Figure 3 where kinases inhibited by a minimum of 80% are shown. A full list of the kinases tested is shown on Table S1 in supplementary information.
Figure 3.
Selectivity profile of compound 55 evaluated on 486 kinases at 1 μM in duplicate (SelectScreen Whole Panel, Life Technologies) and represented on a dendrogram (courtesy of Cell Signalling Technology). Kinases whose activities are inhibited by 80% and above are shown as dots, Haspin is visualised as a green dot, CLKs as purple dots and DYRKs as orange dots.
Selectivity profile of compound 55 evaluated on 486 kinases at 1 μM in duplicate (SelectScreen Whole Panel, Life Technologies) and represented on a dendrogram (courtesy of Cell Signalling Technology). Kinases whose activities are inhibited by 80% and above are shown as dots, Haspin is visualised as a green dot, CLKs as purple dots and DYRKs as orange dots.The inhibitory activities of compound 55 on Haspin, CLKs and DYRKs are well found in this new screening study. Product 55 is not specific but appears to be relatively selective since the compound 55 (AS-N14) presents a reasonable selectivity profile against a panel of 486 tested kinases since it inhibits 73 of the 486 kinases by >80%, and 159 of the 486 kinases by >50% at a dose of 1 µM.
Molecular docking studies
Molecular docking studies were carried out using Glide from the Schrödinger Suite, in order to compare putative binding modes and explore interactions within the active sites of CLK1, DYRK1A and Haspin kinases. Active sites of the three crystal structures were superimposed and are shown in Figure 4. The residues engaging hydrogen bond interactions with docked ligands are highlighted in stick form.
Figure 4.
Superimposition of the ATP site of the three protein kinases, CLK1, DYRK1A and Haspin (residues and ribbons are coloured regarding their localisation in the kinase structure: hinge region (yellow), DFG motif (cyan), G loop (green), Catalytic K (orange), αC-helix (purple) and HRD region (red)), drawn with MOE software. Non-polar hydrogen atoms are hidden for clarity. Catalytic lysine and residues in the hinge region forming hydrogen bonds with the ligand are highlighted. CLK1: Leu244 and Lys191, DYRK1A: Leu241 and Lys188, and Haspin: Gly608, Gly609 and Lys 511.
Superimposition of the ATP site of the three protein kinases, CLK1, DYRK1A and Haspin (residues and ribbons are coloured regarding their localisation in the kinase structure: hinge region (yellow), DFG motif (cyan), G loop (green), Catalytic K (orange), αC-helix (purple) and HRD region (red)), drawn with MOE software. Non-polar hydrogen atoms are hidden for clarity. Catalytic lysine and residues in the hinge region forming hydrogen bonds with the ligand are highlighted. CLK1: Leu244 and Lys191, DYRK1A: Leu241 and Lys188, and Haspin: Gly608, Gly609 and Lys 511.One of the most active compounds, 49 was docked in each active site of the three kinases. The docking poses exhibited the same putative binding mode, highlighting a hydrogen bond between the acceptor atom O of the lactam ring of 49 and the backbone of the hinge Leu244 (CLK1), Leu241 (DYRK1A) and Gly608 (Haspin). In addition, 49 formed another interaction with the hinge region of Haspin through a hydrogen bond between NH of the lactam ring and the backbone of Gly609 (Figure 4). In some docking poses, the molecule was flipped by 180° exposing the methoxy group of 49 towards the solvent area.Derivatives 51 and 62 were next docked in order to investigate the studied binding mode in greater depth since 62 has an N-methyl group on the pyrrole moiety. The best docking poses of the two compounds 51 and 62 were similar to 49 (Figure 5). No steric clash between the protein and the second methoxy group of the ligand was observed. Interestingly, 62 compared to 51 showed a weak H-pi interaction between the methyl group of the indole moiety and the gatekeeper, Phe605, of the kinase. The presence of the methyl group in 62 did not impact the binding mode of the compound, which explains the acceptable IC50 of 62.
Figure 5.
Binding mode representation of 49 (green) and 62 (purple) in ATP site of Haspin. Hydrogen bond interactions are represented in dashed lines.
Binding mode representation of 49 (green) and 62 (purple) in ATP site of Haspin. Hydrogen bond interactions are represented in dashed lines.From the docking experiments, we predicted that the binding mode in each protein kinase, Haspin, CLK1 and DYRK1A, would be very similar. Nevertheless, as in most docking experiments, the docking score is not sufficient to predict the small variation in activity of the compounds and further intensive computational approaches such as free energy of binding (FEB) would be needed.
Cell assays
We next analysed the effects of selected compounds (Haspin IC50 <15 nM) on the cell viability of several cell lines from osteosarcoma (U-2 OS), colorectal cancer (HCT116), breast cancer (MDA-MB231) and neuroblastoma (SH-SY5Y) as well as retinal fibroblast RPE-1 immortalised with hTERT (Figure 6). In a primary screen, all compounds were tested in triplicate at 25 μM and viability was expressed as percentage of a DMSO control. U-2 OS and HCT116 cell lines appeared to be the most sensitive to our compounds and were even slightly more affected than the non-cancerous RPE-1 cell line, whereas the SH-SY5Y and MDA-MB231 cell lines emerged as the most resistant ones. Compounds 46, 49, 51, 54, and 56 had little to no effect on all the tested cell lines. This can be explained by the low solubility of the compounds, or their low affinity for lipidic plasma membrane or a high metabolisation rate in aqueous solution/cellular environment. On the other hand, several compounds such as 48, 61, 55, and 50 showed a reduction of equal or more than 75% of cell viability compared to the DMSO control.
Figure 6.
Effects of compounds on cell viability. Cell viability was assessed on the following human cell lines: U-2 OS (osteosarcoma), HCT116 (colorectal cancer), MDA-MB231 (breast cancer), SH-SY5Y (neuroblastoma) and RPE-1 (retinal fibroblast immortalised with hTERT). Cells were incubated with 25 μM of selected compounds or 10 μM of staurosporine or 0.1% of DMSO for 48 h. Cell viability was evaluated in triplicate via MST assay and results expressed as percentage of DMSO control (mean set at 100%). Results on graphs are mean ± SD.
Effects of compounds on cell viability. Cell viability was assessed on the following human cell lines: U-2 OS (osteosarcoma), HCT116 (colorectal cancer), MDA-MB231 (breast cancer), SH-SY5Y (neuroblastoma) and RPE-1 (retinal fibroblast immortalised with hTERT). Cells were incubated with 25 μM of selected compounds or 10 μM of staurosporine or 0.1% of DMSO for 48 h. Cell viability was evaluated in triplicate via MST assay and results expressed as percentage of DMSO control (mean set at 100%). Results on graphs are mean ± SD.Hence, dose-response experiments were carried out on both U-2 OS and RPE-1 cell lines and EC50 were calculated (Table 5). The results confirmed the lack of efficacy of compounds 46, 49, 54, and 56 which showed EC50 >25 μM on both cell lines regardless of their activity on Haspin kinase (IC50 of 7, 1, 4 and 14 nM respectively). Derivative 51, despite no effect observed on RPE-1 cells (EC50 >25 μM), showed a moderate activity on cell viability of the U-2 OS line with an EC50 of 12.6 μM. The compounds were generally more efficient at inhibiting the viability of U-2 OS cancerous cells than that of normal RPE-1. Amongst the selected compounds, 55 and 50 displayed the strongest effect on the viability of U-2 OS cells (EC50 of 3.4 and 4.3 μM, respectively). They were between 2 and 5 times more active on U-2 OS compared to RPE-1 cell viability.
Table 5.
Effects on cell viability, EC50 on RPE1 and U-2 OS cell linesa.
Entry
Compound
RPE1EC50 in µM
U-2 OSEC50 in µM
1
46
>25
>25
2
48
7.3
7
3
49
>25
>25
4
50
20.8
4.3
5
51
>25
12.6
6
54
>25
>25
7
55
10.7
3.4
8
56
>25
>25
9
61
19.1
8.7
aCells were incubated with increasing doses of each compound (up to 50 µM) for 48 h. Cell viability was determined by MTS assay in triplicate and EC50 (µM) were calculated from the dose-response curves.
Taken together, these results showed that some of our compounds such as 55 and 50 displayed interesting effects on cell viability of several cancerous cell lines.We further examined the effect of our most efficient compound (55) on cancerous cells growing in 3D spheroids. U-2 OS and HCT116 cells spheroids were prepared and treated with different concentrations of either compound 55, CHR-6494 or SBS018 (compound 21 in ref Elie et al) or with 0.5% DMSO for 7 days, after which, spheroids viability was evaluated (Figure 7). We observed a marked dose-dependent effect of compound 55 on both U-2 OS and HCT116 spheroid cell viability after 7 days of treatment. This effect was milder than the one observed with CHR-6494 and stronger than the one induced by SBS018 at similar concentrations.
Figure 7.
Effects of compounds on U-2 OS and HCT116 spheroid viability. Cell viability in spheroids from U-2 OS and HCT116 cells was measured after 7 days of treatment with DMSO (0.5%), CHR6494 (CHR), SBS018 or Cpd55 at a single dose of 2.5, 5, and 10 µM, on day 0. Cell viability is expressed in percentage of the DMSO control. n = 3, results are mean ± s.e.m.
Effects of compounds on U-2 OS and HCT116 spheroid viability. Cell viability in spheroids from U-2 OS and HCT116 cells was measured after 7 days of treatment with DMSO (0.5%), CHR6494 (CHR), SBS018 or Cpd55 at a single dose of 2.5, 5, and 10 µM, on day 0. Cell viability is expressed in percentage of the DMSO control. n = 3, results are mean ± s.e.m.We further characterised the functional effects of our most efficient compound 55 on endogenous Haspin in U-2 OS cells by immunofluorescence, quantifying the Haspin specific H3T3ph signal in early mitotic cells. The H3T3ph signal was measured on cells treated with 0.5 µM of compound 55 or CHR-6494 or SBS018 or with 0.1% of DMSO for 16 h (Figure 8). Our results showed that compound 55 could inhibit intracellular Haspin with a very similar efficiency to that off CHR-6494 or SBS018. These results further validate the functionality of our compound in cells, on the endogenous Haspin kinase activity.
Figure 8.
Cellular endogenous Haspin inhibition. U-2 OS cells were treated for 16 h with 0.5 µM of each compound or 0.1% of DMSO (CHR: CHR-6494). Haspin activity was monitored by immunofluorescence staining of phosphorylated Histone H3 on threonine 3 (H3T3ph, green); α-Tubulin was visualised in red and DNA was stained by DAPI (blue). Haspin activity was quantified in prometaphase/metaphase cells measuring the H3T3ph and DAPI signals and representing the H3T3ph/DAPI ratio on a scatter plot (upper panel). The inserted dot plot allows the comparison of the 3 tested compounds on a more precise scale; n ≥ 15, *p ≤ 0.05; **p ≤ 0.01 (two-tailed unpaired t-test). Representative images are presented on the lower panel, Bar 5 µm.
Cellular endogenous Haspin inhibition. U-2 OS cells were treated for 16 h with 0.5 µM of each compound or 0.1% of DMSO (CHR: CHR-6494). Haspin activity was monitored by immunofluorescence staining of phosphorylated Histone H3 on threonine 3 (H3T3ph, green); α-Tubulin was visualised in red and DNA was stained by DAPI (blue). Haspin activity was quantified in prometaphase/metaphase cells measuring the H3T3ph and DAPI signals and representing the H3T3ph/DAPI ratio on a scatter plot (upper panel). The inserted dot plot allows the comparison of the 3 tested compounds on a more precise scale; n ≥ 15, *p ≤ 0.05; **p ≤ 0.01 (two-tailed unpaired t-test). Representative images are presented on the lower panel, Bar 5 µm.We then characterised the effect of compound 55 on the cell cycle on U-2 OS cells. Cells were treated for 24 h with 1 µM of compound 55, CHR-6494, SBS018 or DMSO at 0.2% and their cell cycle profile was analysed by flow cytometry (Figure 9). Analysis of flow cytometry profiles showed, as expected, a strong increase in the percentage of cells in G2/M phase of the cell cycle with compound 55 as well as with the two references CHR-6494 and SBS018 compared to the DMSO control (20, 17, and 14%, respectively vs. 6% for the DMSO control). Concomitantly, compound 55 further induced a reduction of cells in the G1 phase compared to the control (36 vs. 50%, respectively), an expected result of the strong observed G2/M delay. These results are consistent with an impaired Haspin function inducing prolonged mitoses as previously described (Huertas et al. 2012; Peiling Wang et al. 2021/PMID:34551143).
Figure 9.
Effect of compounds on the cell cycle. U-2 OS cells were treated for 24 h with 1 µM of each compound or 0.2% DMSO (CHR: CHR-6494). DNA content was measured by flow cytometry and the percentages of cells in each phase of the cell cycle is represented on a proportional bar graph. Representative profiles for each treatment are shown on the right panels.
Effect of compounds on the cell cycle. U-2 OS cells were treated for 24 h with 1 µM of each compound or 0.2% DMSO (CHR: CHR-6494). DNA content was measured by flow cytometry and the percentages of cells in each phase of the cell cycle is represented on a proportional bar graph. Representative profiles for each treatment are shown on the right panels.
Conclusion
We have synthesised a series of new Lamellarin analogues using the indolo[2,3-c]quinolone-6-one core. The analogues were obtained after a sequence involving (i) a palladium catalysed cross coupling reaction between 2-indolic esters and 2-nitrophenyl boronic acids as building blocks, and (ii) a cyclic lactam formation involving a reduction and an annelation. Twenty-two novel derivatives were synthesised and evaluated for their inhibitory activity on Haspin kinase and on a panel of 7 other protein kinases for selectivity assessment. Among this series, 8 compounds inhibited Haspin kinase with IC50 below 10 nM. Docking studies showed a double hydrogen bond between the lactam and the hinge region of the kinase. The most active compounds 49 and 55 possess IC50 of 1 and 2 nM respectively with selectivity towards the parent kinases DYRK1A and CLK1 between a 13 and 65-fold factor. Furthermore, the most selective compound 55 exerted an interesting cellular effect on the osteosarcoma U-2 OS cell line as well as on U-2 OS and colorectal carcinoma HTC116 spheroid viability. Additionally, we further validated the functionality of compound 55 on endogenous Haspin activity in cells. This interesting Haspin inhibitor will be used in further studies to develop efficient and selective Haspin inhibitors.
Experimental section
Chemistry
All reagents and solvents were purchased from commercial sources and used without further purification.1H NMR and 13 C NMR spectra were recorded on 400 MHz and/or 500 MHz Bruker FT-NMR spectrometers. All chemical shifts are given as δ values (ppm) with reference to tetramethylsilane (TMS = 0) as an internal standard. The peak patterns are indicated as follows: s, singlet; d, doublet; t, triplet; m, multiplet; q, quartette. The coupling constants, J, are reported in Hertz (Hz). UV detection at 210 nm. High resolution mass (MS) analysis was conducted using an LC/MSD TOF spectrometer system with electrospray ionisation (ESI). Reactions were monitored via thin-layer chromatography (TLC) carried out on commercial silica gel plates (GF254) under UV light. Column chromatography was performed on silica gel 60 (200–300 mesh).
General procedure A: preparation of 3-iodoindoles (11–13)
Indole-2-carboxylic acid derivatives (3.1 mmol) were dissolved in Ethanol (50 ml) and conc. sulphuric acid (5 ml) was added. The solution was refluxed for about 12 h (monitoring with TLC) after completion of the reaction. The solution was poured into cold water (150 ml), and the white solid precipitate formed was collected by filtration. The solid material was washed with water and dried to produce quantitatively derivatives 6–9. Crude materials were next dissolved in a mixture containing crushed KOH (4.0 equiv.) pellets in DMF (15 ml) at room temperature. Next Iodine (1.5 equiv.) dissolved in DMF (3 ml) was added dropwise and the mixture stirred for 4 h at room temperature (monitored with TLC). After completion (TLC monitoring), the reaction mixture was poured onto a saturated aqueous solution of NaHSO3 (15 ml), NH4OH (30%, 2 ml) and water (15 ml). The solid was filtered, dried under reduced pressure, and used directly without further purification. All spectral data for 10, 11, 13 are in agreement with previous reports [20, 21]. Compounds 11–13 were engaged immediately in the next step.
Compound 11 (1.0 g, 2.9 mmol) was added to a stirred suspension of oil-free sodium hydride NaH (0.1 g, 4.36 mmol) in DMF (10 ml) at 0 °C and the mixture was stirred for 10 min at this temperature. Then methyl iodide (0.49 g, 3.48 mmol) was added at 0 °C and the whole mixture was stirred at room temperature (20 °C) for 1 h. The solution was poured into ice cold water (50 ml) and extracted with CH2Cl2 (2 × 25 ml). The organic layers were dried with sodium sulphate and concentrated under reduced pressure to give 14 in a quantitative yield (1.0 g). 1H NMR (CDCl3, 400 MHz) 1.24 (t, J = 7.2 Hz, 3H), 3.95 (s, 3H), 3.81 (s, 3H), 4.28 (q, J = 7.2 Hz, 2H), 7.23 (d, J = 7.4 Hz, 1H), 7.26 (d, J = 7.4 Hz, 1H), 7.64 (s, 1H). 13 C NMR (CDCl3, 125 MHz) 14.6, 33.6, 55.9, 61.5, 66.5, 103.2, 113.2, 117.9, 129.2, 130.4, 134.5, 155.6, 161.1; ESI-MS m/z 360 [M + H]+; IR (KBr) ν 2995, 2826, 1701, 1573–1454, 767 cm−1.
General Procedure B: synthesis of 2-nitrophenyl boronic acids (15–20)
A dry nitrogen-flushed 25-ml round-bottomed flask equipped with a magnetic stirrer and a septum was loaded with aryl iodide (4.0 mmol, 1.0 equiv.). Dry THF (6 ml) was added, and the resulting solution was cooled to −78 °C. To the resulting cooled mixture was added dropwise 2.2 ml of a 2 M solution of PhMgCl (4.8 mmol, 1.2 equiv.) in THF. After 5 min, 0.536 ml of trimethyl borate (4.8 mmol, 1.2 equiv.) was added dropwise to the reaction solution. The reaction mixture was stirred for 30 min at −78 °C, warmed to −10 °C and quenched with 4 ml of a 2 M aqueous solution of HCl. The resulting mixture was extracted with Et2O (20 ml) and washed with H2O (10 ml) and brine (10 ml). The resulting organic layer was dried over Na2SO4, filtered, and concentrated under reduced pressure. The crude boronic acids were used in subsequent transformations without additional purification.
General Procedure C: synthesis of 2-nitrophenyl boronic esters (21–24)
In a 250-ml round-bottomed flask purged and maintained with an inert atmosphere of nitrogen was placed a solution of substituted-1-bromo-2-nitrobenzene (1.0 equiv.) in 1,4-dioxane (150 ml). Bis(pinacolato)diboron (1.5 equiv.), Pd(dppf)Cl2 (0.03 equiv.), and potassium acetate (2.0 equiv.) were then added under vigorous stirring and placed in a heated bath at 80 °C. The resulting solution was stirred overnight, cooled to room temperature and concentrated under reduced pressure. The residue was used for further steps without purification.
General procedure D: synthesis of 3-arylated indoles (25–44)
To a mixture of ethyl 3-iodo-5- or 6-substituted-1H-Indole-2-carboxylate 10–14 (1.0 equiv.), crude substituted-2-nitroarylboronic acid 15–20 or 4,4,5,5-tetramethyl-2-(substited-2-nitrophenyl)-1,3,2-dioxaborolane 21–24 (2.0 equiv.) and finally sodium bicarbonate (3.0 equiv.) was added a 10:1 v/v mixture of 1,4-dioxane and water. The reaction mixture was degassed with argon for about 30 min and Pd(PPh3)4 (10.0 mol %) was added in one portion. The resulting mixture was heated to 100 °C. After 12 h, the mixture was cooled to room temperature and diluted with cold water. The mixture was extracted with EtOAc. The combined organic layers were washed with brine, dried over Na2SO4, filtered and concentrated in vacuo. The crude product was finally purified by silica gel flash chromatography to afford the desired product 25–44.
The reaction was carried out as described in general procedure C using 14 (0.100 g, 0.278 mmol, 1.0 equiv.) and (2-(dimethylamino)-5-nitrophenyl)boronic acid 20 (0.117 g, 0.557 mmol, 2.0 equiv.). Purification by flash chromatography on silica gel (eluent 9/1 PE/EtOAc) afforded 44 (0.072 g, 65%) as a yellow solid, which was used in the next step. Rf = 0.5 (PE/EtOAc 8/2). 1H NMR (CDCl3, 400 MHz) 1.00 (t, J = 7.2 Hz, 3H), 3.07 (s, 6H), 3.75 (s, 3H), 4.05–4.11 (m, 5H), 6.55 (d, J = 2.8 Hz, 1H), 6.66 (dd, J = 2.8 Hz, 9.2 Hz, 1H), 6.76 (d, J = 2.4 Hz, 1H), 7.05 (dd, J = 2.4 Hz, 8.8 Hz, 1H), 7.33 (d, J = 8.8 Hz, 1H), 8.19 (d, J = 9.2 Hz, 1H). ESI-MS m/z 398 [M + H]+. IR (KBr) ν 3045, 2980, 2928, 1701, 1612, 1515, 1403,1241,1107,1032, 975,729 cm−1.
General procedure D: synthesis of the indolo[2,3-c]quinolin-6-one library 45–64
Ethyl 3-(substituted-2-nitrophenyl)-1H-substituted-indole-2-carboxylate 25–44 (1.0 equiv.) was dissolved in acetic acid and Iron (Fe) powder (5.0 equiv.) was added. The reaction mixture was heated to 110 °C for about 12 h. After completion of the reaction, the acetic acid was removed under reduced pressure and the residue was diluted with EtOAc. After filtration and evaporation under reduced pressure, the crude material was purified by silica gel flash chromatography (CH3OH/CH2Cl2).
5,7-Dihydro-6H-indolo[2,3-c]quinolin-6-one (45)
The reaction was carried out as described in general procedure D using 25 (0.090 g, 0.29 mmol, 1.0 equiv.). Purification by flash chromatography on silica gel (eluent 9/1 CH2Cl2/MeOH) afforded 45 (0.054 g, 80%) as a white solid. Rf = 0.5 (5% CH3OH in CH2Cl2). mp 233–237 °C. 1H NMR (DMSO-d6, 400 MHz) 7.31–7.36 (m, 2H), 7.42(d, J = 7.6 Hz, 1H) 7.46–7.53(m, 2H), 7.65(d, J = 8 Hz, 1H), 8.45 (d, J = 7.6 Hz, 1H), 8.48 (d, J = 8.0 Hz, 1H), 11.87 (s, 1H, Imid-NH), 12.37 (s, 1H, amide-NH).13C NMR (DMSO-d6, 125 MHz) 113.5, 116.5, 118.5, 118.7, 121.1, 122.7, 122.8, 123.4, 126.1, 126.3, 128.1, 135.4, 139.3, 156.2. ESI-MS m/z 235 [M + H]+. HRMS (TOF-MS): m/z calcd for C15H11N2O [M + H]+: 235.0871, found: 235.0861; IR(KBr) ν 3319, 3157, 3004, 1655, 1621, 1594, 1254, 731 cm−1.
The reaction was carried out as described in general procedure D using 32 (0.060 g, 0.15 mmol, 1.0 equiv). The crude mixture was purified by flash chromatography on silica gel (eluent 9/1 CH2Cl2/MeOH) to afford 52 (0.031 g, 65%) as a white solid. This compound was not soluble enough to provide a correct 13 C NMR spectrum. Rf = 0.4 (5% CH3OH in CH2Cl2). mp 205–208 °C. 1H NMR (DMSO-d6, 400 MHz) 3.82 (s, 3H), 3.91 (s, 3H), 3.97 (s, 3H), 7.10 (s, 1H), 7.13 (s, 1H), 7.51 (s, 1H), 7.72 (d, J = 12.4 Hz, 2H), 11.57 (s, 1H), 12.01 (s, 1H); ESI-MS m/z 325 [M + H]+. HRMS (TOF-MS): m/z calcd for C18H16N2O4 [M + H]+: 325.1188, found: 325.1182. IR (KBr) ν 3259, 3161, 3024,2982, 2920, 1667, 1621, 1575, 1234,1205, 1102, 747 cm−1.
The reaction was carried out as described in general procedure D using 44 (0.065 g, 0.163 mmol, 1.0 equiv.). The crude mixture was purified by flash chromatography on silica gel (eluent 9/1 CH2Cl2/MeOH) to afford 64 (0.039 g, 75%) as a white solid. Rf = 0.7 (5% CH3OH in DCM). mp 231–234 0 C. 1H NMR (DMSO-d6, 400 MHz) 3.00 (s, 6H), 3.91 (s, 3H), 4.28 (s, 3H), 6.94 (dd, J = 2.4 Hz, 8.8 Hz, 1H), 7.21 (dd, J = 9.2 Hz, 2.4 Hz, 1H), 7.31 (d, J = 9.2 Hz, 1H), 7.44 (d, J = 2.4 Hz, 1H), 7.65 (d, J = 8.8 Hz, 1H), 7.16 (d, J = 2.4 Hz, 1H), 11.51 (s, 1H). 13 C NMR (DMSO-d6, 125 MHz) 31.7, 41.2, 55.9, 103.9, 104.9, 112.4, 113.6, 116.2, 116.9, 118.3, 119.2, 121.9, 126.9, 127.3, 135.9, 146.9, 154.8, 156.1; ESI-MS: m/z 322 [M + H]+. HRMS (TOF-MS). m/z calcd for C19H20N3O2 [M + H]+: 322.1556, found: 322.1555. IR (KBr) ν 3145, 3020, 2950, 2910, 1675, 1600, 1564, 1210, 754 cm−1.
Cell culture
HCT116 cells were cultured in McCoy’s medium. SH-SY5Y, MDA-MB231 and U-2 OS cells were cultured in Dulbecco's modified Eagle's medium (DMEM) and hTERT RPE-1 cells in DMEM:F12 medium. All media were supplemented with 10% foetal calf serum and cells were cultured at 37 °C in a 5% CO2 humidified atmosphere.
Cell viability
Cells were grown in 96-well plates in the presence of a fixed concentration of 25 μM of each compound (for cell viability primary assessment) or increasing concentrations of each compound (from 50 to 0.05 µM) for 48 h (for EC50 determination). Cell viability was then assessed using the CellTiter96 AQueous cell proliferation assay from Promega according to the manufacturer’s instructions. Each experiment was done in triplicate and EC50 were determined from the dose-response curves according to the signal given by the control (0.1% DMSO) set at 100% viability using Prism GraphPad software.
3D Spheroid viability
U-2 OS cells were seeded at 5000 cells per well and HCT116 at 1500 cells per well, in 96-well black ULA plates (Ultra Low Adherence, Corning). After centrifugation at 200 g for 10 min, spheroids were incubated at 37 °C for 3 days in order to reach 400 µm in diameter. Compounds were then added at a single dose (2.5, 5, or 10 μM) and cell viability was measured after 7 days using the CellTiter-Glo® 3D Cell Viability Assay (Promega) following the manufacturer's protocol. Luminescence was measured using an EnVision® plate reader (Perkin Elmer).
Endogenous haspin activity measurement
U-2 OS cells were grown on glass coverslips, treated for 16 h than fixed with 4% paraformaldehyde in PBS, permeabilized by 0.15% Triton-X100 for 2 min, blocked for 15 min in 4% BSA in PBS and processed using standard immunofluorescence protocols. Primary antibodies included anti-phospho-Thr3 Histone H3 (1/1000 dilution, Millipore) and anti-α-tubulin (1/5000 dilution, clone B512, Sigma). Images were acquired with a Coolsnap HQ2 CCD camera (Photometrics) on a Zeiss Axio microscope (Carl Zeiss) using a 63x NA 1.40 objective. Image acquisition and processing were performed using Metamorph (Molecular Device). Quantification of signal intensity was performed using ImageJ software (NIH).
Cell cycle analysis
After treatment with the compounds, cells were trypsinized and washed once in PBS. Cells were fixed for 1 h in ice-cold 70% ethanol, then washed once in PBS, centrifuged at 200 g and resuspended in a PBS buffer containing 100 µg/ml RNase A (Thermo Scientific) and 40 µg/ml propidium iodide (Life Technologies). DNA content was determined using a flow cytometer AttuneTM NxT (Thermofisher) and ten thousand events were collected in each run. The data were analysed using FCS Express 7 Pro software (De Novo).
Kinase assays
Kinase activities were determined using the ADP-Glo methodology (ADP-Glo Kinase Assay; Promega) according to the assay described by Nguyen et al. except for MmCLK1. The later was assayed in the following buffer: 10 mM MgCl2, 1 mM EGTA, 1 mM DTT, 25 mM Tris-HCl pH 7.5, 50 µg/ml heparin, 0.15 mg/ml BSA, with 0.027 µg/µl of the following peptide: GRSRSRSRSRSR as substrate.
Molecular modelling
Structure preparation
Marvin was used for drawing chemical structures. Structures were prepared with VSPrep, a workflow dedicated to the preparation of ligands for virtual screening, and finally given as input to Glide, the docking software from the Schrödinger Molecular Modelling Suite 2019–0131. Structural data of CKL1 kinase complexed with a methyl 9-anilinothiazolo[5,4-f] quinazoline-2-carbimidate (EHT1610) compound were retrieved from the protein data bank, PDB entry 6YTI (unpublished data). DYRK1A in complex with a pyrido[2,3-d]pyrimidine inhibitor, the N-(5-([(1R)-3-amino-1–(3-chlorophenyl)propyl]carbamoyl)-2-chlorophenyl)-2-methoxy-7-oxo-7,8-dihydropyrido[2,3-d]pyrimidine-6-carboxamide, was retrieved from the protein data bank, PDB entry 4MQ1. Structural data of Haspin kinase complexed with an imidazo[1,2-b]pyridazine derivative compound were retrieved from the protein data bank, PDB entry 3F2N (unpublished data). The three high-resolution crystal structures of CLK1, DYRK1A and Haspin were superimposed before carrying out molecular docking experiments. All the receptors were prepared using the Protein Preparation Wizard workflow from the Schrödinger Molecular Modelling Suite 2019–01. Hydrogen atoms were added, water molecules were removed, the hydrogen network automatically was optimised and finally proteins were minimised (OLPS2005 force field) with a convergence criterion of RMSD on heavy atoms of 0.3 Å (other parameters were fixed to their default values).
Docking parameters
Docking grids were centred and sized on crystalised ligands. Docking calculations were performed with extra precision. Ligand flexibility was considered and the option of sampling of ring conformation was activated. A maximum of 100 poses were generated and a post-docking minimisation was performed.We have synthesised a series of new Lamellarin analogues using the indolo[2,3-c]quinolone-6-one core. The analogues were obtained after a sequence involving (i) a palladium catalysed cross coupling reaction between 2-indolic esters and 2-nitrophenyl boronic acids as building blocks, and (ii) a cyclic lactam formation involving a reduction and an annelation. Twenty-two novel derivatives were synthesised and evaluated for their inhibitory activity on Haspin kinase and on a panel of 7 other protein kinases for selectivity assessment. Among this series, 8 compounds inhibited Haspin kinase with IC50 below 10 nM. Docking studies showed a double hydrogen bond between the lactam and the hinge region of the kinase. The most active compounds 49 and 55 possess IC50 of 1 and 2 nM respectively with selectivity towards the parent kinases DYRK1A and CLK1 between a 13 and 65-fold factor. Furthermore, the most selective compound 55 exerted an interesting cellular effect on the osteosarcoma U-2 OS cell line as well as on U-2 OS and colorectal carcinoma HTC116 spheroid viability. Additionally, we further validated the functionality of compound 55 on endogenous Haspin activity in cells. This interesting Haspin inhibitor will be used in further studies to develop efficient and selective Haspin inhibitors.Click here for additional data file.
Authors: Wolfgang Wick; Vinay K Puduvalli; Marc C Chamberlain; Martin J van den Bent; Antoine F Carpentier; Lawrence M Cher; Warren Mason; Michael Weller; Shengyan Hong; Luna Musib; Astra M Liepa; Donald E Thornton; Howard A Fine Journal: J Clin Oncol Date: 2010-02-01 Impact factor: 44.544
Authors: Elizabeth O Hexner; Cynthia Serdikoff; Mahfuza Jan; Cezary R Swider; Candy Robinson; Shi Yang; Thelma Angeles; Stephen G Emerson; Martin Carroll; Bruce Ruggeri; Pawel Dobrzanski Journal: Blood Date: 2007-11-05 Impact factor: 22.113
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