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Antiradical, antimicrobial and enzyme inhibition evaluation of sulfonamide derived esters; synthesis, X-Ray analysis and DFT studies
Accepted Manuscript Antiradical, Antimicrobial and Enzyme Inhibition Evaluation of Sulfonamide Derived Esters; Synthesis, X-Ray Analysis and DFT Studies
Muhammad Danish, Ayesha Bibi, Khola Gilani, Muhammad Asam Raza, Muhammad Ashfaq, Muhammad Nadeem Arshad, Abdullah Mohamed Asiri, Khurshid Ayub PII:
S0022-2860(18)30943-8
DOI:
10.1016/j.molstruc.2018.07.116
Reference:
MOLSTR 25521
To appear in:
Journal of Molecular Structure
Received Date:
01 June 2018
Accepted Date:
31 July 2018
Please cite this article as: Muhammad Danish, Ayesha Bibi, Khola Gilani, Muhammad Asam Raza, Muhammad Ashfaq, Muhammad Nadeem Arshad, Abdullah Mohamed Asiri, Khurshid Ayub, Antiradical, Antimicrobial and Enzyme Inhibition Evaluation of Sulfonamide Derived Esters; Synthesis, X-Ray Analysis and DFT Studies, Journal of Molecular Structure (2018), doi: 10.1016/j. molstruc.2018.07.116
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ACCEPTED MANUSCRIPT
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Antiradical, Antimicrobial and Enzyme Inhibition Evaluation of Sulfonamide Derived
2
Esters; Synthesis, X-Ray Analysis and DFT Studies
3
Muhammad Danisha*, Ayesha Bibia, Khola Gilania, Muhammad Asam Razaa, Muhammad
4
Ashfaqa, Muhammad Nadeem Arshadb, Abdullah Mohamed Asirib*, Khurshid Ayubc aDepartment
5 6
bChemistry
Department, Faculty of Science, King Abdulaziz University, Jeddah 21589, Saudi Arabia
7 8
of Chemistry, University of Gujrat, Gujrat 50700 Pakistan
cDepartment
of Chemistry, COMSATS Institute of Information Technology, Abbottabad, KPK,
9
Pakistan, 22060
10
Authors for correspondence:[email protected], [email protected]
11 12
Abstract
13
Two carboxylate esters (methyl: (I) and ethyl: (II)) of 4-{(4-methylphenylsulfonamido)-
14
methyl}cyclohexanecarboxylic acid (sulfonamide) were synthesized and characterized by FTIR
15
and X-ray crystallography. DFT studies were conducted in order to optimize the structures using
16
Gaussian software which confirmed the bond angels and bond lengths obtained from single
17
crystal analysis. Both Compounds (I and II) were evaluated for their biological studies viz;
18
antioxidant activity (DPPH ), enzyme inhibition activity (esterase and proteases), antibacterial
19
(Halomonas halophila, Halomonas salina, Shigella sonnei, Bacillus subtilis, Chromohalobacter
20
salexigens, Chromohalobacter israelensis, Staphylococcus aureus, Escherichia coli and
21
Klebsiella pneumoniae) and anti-fungal (Aspergillus niger and Alternaria alternata). Results
22
depicted that II is more active as compared to I in antioxidant and esterases while I is more
23
potent against protease while moderate results were shown by both.
24
Keywords: Antioxidant; DFT; Enzyme Inhibition; Ester;. Sulfonamide. .
25 26 27
1.
Introduction
28
Sulfonamides have been found to show broad pharmacological profile. They are stable in human
29
body and being used for the treatment of various diseases i.e. tumor, diabetes and other major 1|Page
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pathogens. Moreover, they are used in agriculture field as well as insecticides and herbicides.
31
They are less toxic as compared to other drugs and are scalable
32
that minor variation in the structure of sulfonamide gives vast range of applications both
33
qualitatively as well as quantitatively. Sulfonamides have been proved to be wonderful drugs as
34
they serve the humanity meritoriously for health e.g. as antitumor, antibacterial, antifungal and
35
inhibition against lipoxygenase enzyme [4-7]. As β3 adrenergic agonist, they serve for the
36
treatment of obesity and type 2 diabetes [8-10]. The biological potential of the sulfonamides
37
depends to which way, they attach to their respective receptor or enzyme. This aptitude of
38
binding depends upon proton-ligand complex of the sulfonamides [11]. After the discovery of
39
sulfanilamide, so many chemical alteration have been done and evaluated their therapeutic
40
results.
41
following different synthetic schemes. These syntheses have resulted in the finding of new
42
agents with changeable pharmacological properties [12]. Density functional theory (DFT) has
43
long been renowned as a best tool in the understanding of organic complex previous methods
44
used in the past. Detailed analyses on the performance of various DFT methods have been
45
carried out predominantly for the optimized geometry or structure [13]. Keeping in view such
46
therapeutic applications, new esters derived from sulfonamides were synthesized and
47
characterized. Evaluation of these synthesized compounds for their pharmacological profile
48
involving enzyme inhibition, bactericidal, fungicidal and anti-oxidant potential is also part of this
49
research task.
[1-3]. It has been reported
Up-to date greater than 20,000 sulfanilamide derivatives have been synthesized
50 51
2.
Experimental
52
Chemical for this research task were purchased from Alfa Aesar and Merck (UK). Solvents used;
53
Methanol, Ethanol and Dimethyl Sulfoxide of analytical grade were purchased from Merck
54
(UK). Perkin-Elmer System 100 FT-IR spectrophotometer was used for IR spectral data (4000-
55
400 cm-1) while X-ray diffraction analysis was done on Atlas diffractometer.
56
2.1
57
(I) and Ethyl-4-{(4-methylphenylsulfonamido)methyl} cyclohexanecarboxylate (II)
58
10 mL alcohol (methanol and ethanol) was taken in 100 mL round bottom flask and acidified
59
with 1 mL of conc. H2SO4, followed by the addition of 0.5 gram of 4-{(4-
60
methylphenylsulfonamido)methyl}cyclohexanecarboxylic acid. The mixture was refluxed for
Synthesis of Methyl-4-{(4-methylphenylsulfonamido)methyl} cyclohexanecarboxylate
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about 6 hours and stirred overnight at room temperature. After stirring it was concentrated at
62
room temperature via slow evaporation until crystalline product obtained. H3C O
CH3OH
S O
NH
H3C
OCH3
(I)
O S O
O
NH OH
H3C
O
O
C2H5OH
S O
NH OC 2 H5
(II)
63
O
64
2.2
Characterization of the Synthesized Esters
65
Both compounds were characterized on the basis of FTIR and single XRD analysis.
66
2.3
67
Quantum chemical calculations were performed with Gaussian 09 (Revision C.01) [14]. The
68
results are visualized with Gauss View 5.0. The geometries of the compounds are optimized
69
without any symmetry constraints using the hybrid functional B3LYP method 6-31G(d,p) basis
70
set [15]. B3LYP method consists of Becke’s three-parameter (B3) hybrid exchange functional in
71
conjunction with the correlation functional of Lee Yang and Parr (LYP) [16,17]. The basis set
72
chosen contains polarization functions on all atoms. The B3LYP method of DFT is quite reliable
73
for the prediction of geometric and electronic properties of neutral and charged species ranging
74
from simple molecular to polymer structures [18-26]. For optimization, the input geometries are
75
taken from the crystal structure (where available) in order to better match with the
76
experimentally obtained structures. Frequency calculations are also performed at the same level
77
in order to confirm these structures as true minima (absence of an imaginary frequency).
78
2.4
Biological Activities
79
2.4.1
Antimicrobial Assay
DFT studies
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Disc diffusion method was used to measure antimicrobial activity of synthesized compounds
81
against nine bacterial strains; Halomonas halophila, Halomonas salina, Shigella sonnei, Bacillus
82
subtilis, Chromohalobacter salexigens, Chromohalobacter israelensis, Staphylococcus aureus,
83
Escherichia coli, Klebsiella pneumoniae and two fungal strains (Alternaria alternata and
84
Aspergillus niger) according to procedure of Shahid et al., (2009) [27]. Prepared the growth
85
medium, autoclaved at 121oC and transferred 30 mL of this solution to the petri dishes. After
86
solidification of medium, corresponding strain was used to seed medium. 20 µL (5 mg/mL)
87
sample solution was loaded on each disc. Kanamycin, ampicillin and streptomycin were used as
88
reference drugs for bacteria while fungivin was used as antifungal drug. The plates were
89
incubated at 37 oC (24 hours) and 25 oC (48 hours) for bacterial and fungal respectively.
90
2.4.2
91
The methodology of Shahwar et al., (2010) was used to measure the anti-oxidant activity by
92
using radical (2-2’-dienyl-1-picrylhydrazyl) [28]. DPPH solution was prepared in methanol with
93
concentration level of 0.0025g/mL. In first step, added 100µL of each of compound’s sample
94
solution into 2mL DPPH solution in test tube and allowed to stand in darkness for 30 minutes.
95
The absorbance of mixture was recorded at 517 nm keeping methanol was used as blank while
96
Gallic acid was used as standard. % age inhibition was calculated using formula given below.
97
% Inhibition
98
2.4.3
99
Esterases inhibitory activity of synthesized compounds against acetyl cholineesterase (AChE)
100
and butyrylcholine esterase was determined by method of Ellman et al., (1961) along some
101
modifications [29]. 100 μL test compound (5 mg/mL) was mixed with 100 μL enzyme (AChE
102
and BChE) and incubate at 37 °C for 10 minutes. After incubation 0.5 mL buffer (50 mM), 50
103
μL DTNB followed by addition of 50 μL substrate acetylthiocholine iodide and
104
butyrylthiocholine iodide for AChE and BChE respectively. After 30 minutes of incubation at 37
105
°C, the absorbance was measured at 410 nm using UV/VIS spectrophotometer. All experiments
106
were carried out with their respective controls in triplicate. The %age inhibition was calculated
107 108
by the formula mentioned in antioxidant assay.
109
2.4.4
Antioxidant Assay
Absorbance (blank) - Absorbance (test) 100 Absorbance (blank)
Esterases Inhibitory Activity
α-Chymotrypsin Protease Assay 4|Page
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Protease inhibition study of compounds was done by using methodology of Raza, et al., (2013)
111
with minor modifications [30]. In first step, added 100 µL of test sample as well as enzyme,
112
shaked and waited for 10 minutes. 0.5 mL of tris-buffer was added in this solution mixture
113
followed by addition of substrate. Incubation of mixture was done at 37 oC for 30 minutes.
114
Added 0.5 mL distilled water in this solution and recorded the absorbance at 410 nm with UV-
115
VIS spectrophotometer. The %age inhibition was calculated by the formula mentioned in
116
antioxidant assay.
117
3.
118
The sulfonamide was reacted in acidic medium with methanol (I) and ethanol (II) on stirring
119
which resulted white precipitates. The products (I and II) were crystallized in ethanol and
120
characterized with FT-IR and single crystal XRD techniques. In infrared spectra of compounds
121
(I) and (II), the disappearance of broad peak around 3000 cm-1 indicated the deprotonation of
122
acid and formation of ester. Both esters showed the sharper peak in range of 3226 cm-1 (I) to
123
3298 cm-1 (II) indicating the presence of NH group [31]. CH of aliphatic group showed the peak
124
in range of 2922 cm-1 (I) to 2931cm-1 (II). SO2 group gave sharp peaks of the asymmetric and
125
symmetric stretching frequencies in range of 1314 - 1315 cm-1 and 1140 -1146 cm-1 respectively.
126
The stretching frequencies for carboxylate group (COO) were given in the range of 1718 cm-1 (I)
127
to 1720 cm-1 (II) for both compounds showing the confirmation of esters moiety in compounds
128
[32].
Result and Discussion
129
The information about the spatial arrangements of molecules (I and II) in the unit cell is
130
very important for their further physico-chemical properties. Samples of crystallized material
131
were screened out under microscope and glued over a glass fiber tip immersed in a wax on
132
copper rod with magnetic base. This holder was mounted on Agilent Super Nova (Dual source)
133
Agilent Technologies Diffractometer, equipped with graphite-monochromatic Cu/Mo Kα
134
radiation for data collection. The data collection was accomplished using CrysAlisPro software
135
at 296 K under the Mo Kα radiation [33]. The structure solution was performed using SHELXS–
136
97 and refined by full–matrix least–squares methods on F2 using SHELXL–97, in-built with
137
WinGX [34,35]. All non–hydrogen atoms were refined anisotropically by full–matrix least
138
squares methods [34]. Figures were drawn using PLATON and ORTEP-3 [36,37].
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139
All the hydrogen atoms attached to the aromatic carbon atoms were positioned geometrically and
140
treated as riding atoms with C–H = 0.93 Å and Uiso(H) = 1.2 Ueq(C) carbon atoms. The N-H =
141
0.85(1) Å, hydrogen atom was located with difference fourier map and refined using the DFIX
142
restraint with Uiso (H) = 1.2 Ueq(O). The methyl and methylene hydrogen atoms were also
143
positioned geometrically with C–H = 0.96 Å and Uiso(H) = 1.5 Ueq(C) for methyl group and C–
144
H = 0.97 Å and Uiso(H) = 1.2 Ueq(C) for methylene hydrogen atoms. The Van der Waals’
145
interactions among the molecules produce extra stability of crystal structures. The compound (I)
146
was crystallized with the emphasis to know internal geometry and Van der Waals’ interaction of
147
the molecules in their crystal structures. The study is in continuation of already reported crystal
148
structures of sulfonamides molecules by our group [38,39]. The presented molecule (Figure 1)
149
was crystallized with monoclinic crystal system and P2 1/n space group Table 1. Hydrogen
150
bonding were shown in Table 2 while selected bond lengths and bond angles are provided in
151
Table 3 and 4 respectively.
152
153 154
Figure 1: ORTEP diagram of molecule I where thermal ellipsoids were drawn at 50%
155
probability level
156 157
The cyclohexane ring adopted the chair shape conformation and the root mean square (r. m. s)
158
deviation for the fitted atoms of this ring is 0.2308 Å. The dihedral angles between the planes of
159
cyclohexane atoms and aromatic ring is 21.55 (1)º which is lesser than its parent molecule 4-{(4-
160
methylbenzenesulfonamido)methyl}cyclohexanecarboxylic acid.23 The puckering parameters for
161
the cyclohexane rings are QT = 0.565 (2) Å, θ = 177.8 (5)°, φ = 188.8 (6)° [40]. Methyl-ester
162
group is twisted with the dihedral angle of 53.20 (1) º with respect to cyclohexane ring. A very 6|Page
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163
beautiful network produced through the intermolecular hydrogen bonding which connects the
164
molecules to form the infinite chains along c-axis [0 0 1] as shown in Figures 2 & 3. Atoms N(1)
165
and C(12) in the molecule situated at (x, y, z) act as hydrogen bond donor via H(1N) and H12, to
166
atoms O(4) and O(1) respectively at (x, y, z-1). Both the interactions produced seventeen
167
membered ring motif R22 [41].
168 169 170 171
Figure 2: Unit Cell Diagram of I, showing intermolecular hydrogen bonding interactions
172
using dashed lines
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173 174
Figure 3: Formation of infinite one-dimensional chains along c-axes through hydrogen
175
bonding
176
The molecule II was crystalized in orthorhombic crystal system and unit cell parameters were a =
177
5.3382(3) Å, b = 9.5791(9) Å, c = 36.078(3) Å, V = 1844.8(3) Å3. The data was collected at T =
178
296.15 K with space group P212121 (no. 19) and Z = 4. The final wR2 was 0.1647 (all data)
179
and R1 was 0.0634 (I > 2\s(I)). In the crystal structure of compound II, the O-S-O angle around
180
the S atom is 120.6(2)º giving rise to formation of distorted tetrahedral geometry, where the
181
corner of tetrahedron are being occupied by the C1, N1, O1 and O2 atoms. The dihedral angle
182
between the aromatic ring and plane produced through the fitted atoms of cyclohexane ring is
183
62.086 (2)º. The root mean square (r.m.s) deviation for the cyclohexane ring observed is 0.2318
184
Å and puckering parameters observed are QT = 0.568 (2) Å, θ = 176.99 (5)°, φ = 6.807 (2)°. The
185
ethyl group is disordered over two positions with the site occupancy of 0.73 and 0.27 for major
186
and minor components. Infinite chains observed, produced through the hydrogen bonding
187
interaction between the N-H and SO2 of sulfonamide group. Atoms N1 in the molecule located at
188
(x, y, z) act as hydrogen bond donor via H1N, to atoms O2 at (x-1, y, z).
189
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190
191
Figure 4: Crystal Structure of II
192 193
194
Figure 5: Packing Diagram of II
195 196 197
Table 1: Crystal Data and Structure Refinement of Compound I and II Crystal Data and Structure
I
Refinement Empirical formula Formula weight
C16H23NO4S 325.41
II C17H25NO4S 339.44
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Temperature/K
296(2)
Crystal system
Monoclinic
Space group
P21/n
296.15 orthorhombic P212121
a/Å
7.9687(12)
5.3382(3)
b/Å
25.817(4)
9.5791(9)
c/Å
8.2971(10)
36.078(3)
α/°
90
89.941(7)
β/°
102.959(13)
89.993(6)
γ/°
90
89.995(6)
1663.5(4)
1844.8(3)
Volume/Å3 Z
4
4
ρcalcmg/mm3
1.299
1.222
μ/mm-1
0.212
0.194
F(000)
696.0
728.0
Crystal size/mm3 2θ range for data collection Index ranges Reflections collected Independent reflections Data/restraints/parameters Goodness-of-fit on F2 Final R indexes [I>=2σ (I)]
0.27 × 0.08 × 0.04 5.946 to 57.958° -8 ≤ h ≤ 10, -24 ≤ k ≤ 35, -10 ≤ l ≤ 11 8267 3903[R(int) = 0.0558] 3903/1/202 0.984 R1 = 0.0694, wR2 =
0.420 × 0.270 × 0.210 6.208 to 59.014° -5 ≤ h ≤ 7, -13 ≤ k ≤ 9, 45 ≤ l ≤ 48 9718 4390[R(int) = 0.0472] 4390/0/213 1.019 R1 = 0.0634, wR2 = 10 | P a g e
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0.1351 Final R indexes [all data]
0.1249
R1 = 0.1491, wR2 =
R1 = 0.1492, wR2 =
0.1770
Largest diff. peak/hole / e Å-3
0.1647 0.22/-0.23
0.18/-0.26
Flack parameter
0.77(18)
198
Table 2: Hydrogen Bonds for Compound I
199
D
A
d(D-H)/Å
C12
H12 O11
0.93
2.58
3.447(4)
156.2
N1
H1N O41
0.858(10)
2.098(19)
2.878(4)
151(3)
1+X,
H
d(H-A)/Å
d(D-A)/Å
D-H-A/°
+Y, -1+Z
200
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Table 3: Bond Lengths of synthesized compounds
202
I Atoms
II
Experimental
Theoretical
Atoms
Length/Å
Experimental
Theoretical
Length/Å 1.539
S1
O1
1.430(4)
1.464
1.525(4)
1.537
S1
O2
1.442(4)
1.464
C7
1.526(4)
1.535
S1
N1
1.617(4)
1.681
C2
C3
1.521(4)
1.535
S1
C1
1.766(6)
1.798
C3
C4
1.538(4)
1.535
O3
C14
1.192(6)
1.213
C4
C5
1.513(5)
1.548
O4
C14
1.323(6)
1.354
C4
C15
1.500(4)
1.518
O4
C15
1.467(7)
1.449
C5
C6
1.524(4)
1.534
N1
C7
1.473(6)
1.468
C7
N1
1.467(4)
1.474
C1
C2
1.373(8)
1.395
C8
C9
1.384(5)
1.397
C1
C6
1.393(7)
1.397
C8
C13
1.388(4)
1.395
C2
C3
1.398(9)
1.394
C8
S1
1.763(3)
1.797
C3
C4
1.367(9)
1.401
C9
C10
1.371(5)
1.391
C4
C5
1.374(9)
1.403
C10 C11
1.392(5)
1.403
C4
C17
1.517(9)
1.509
C11 C12
1.379(5)
1.400
C5
C6
1.379(8)
1.392
C11 C14
1.515(5)
1.509
C7
C8
1.523(6)
1.535
C12 C13
1.387(4)
1.394
C8
C9
1.516(6)
1.540
C15 O3
1.329(4)
1.355
C8
C13
1.528(6)
1.540
C15 O4
1.205(4)
1.212
C9
C10
1.524(6)
1.533
C16 O3
1.450(4)
1.436
C10
C11
1.520(6)
1.534
N1
S1
1.593(3)
1.678
C11
C12
1.532(7)
1.547
O1
S1
1.430(2)
1.464
C11
C14
1.507(6)
1.520
C1
C2
C1
C6
C1
1.517(5)
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O2
S1
1.464
1.438(3)
C12
C13
1.528(6)
1.534
C15
C16
1.347(13)
1.520
203
Table 4: Bond Angles of synthesized compounds
204
I Atom
II
Experimental Theoretical
Experimental Theoretical
Atom
Angle/˚
Angle/˚
C2 C1 C6
109.8(3)
110.36
O1
S1
O2
120.6(3)
122.81
C2 C1 C7
112.1(3)
112.15
O1
S1
N1
106.4(3)
106.43
C6 C1 C7
112.1(3)
110.40
O1
S1
C1
108.3(2)
107.19
C1 C2 C3
111.9(3)
111.87
O2
S1
N1
106.9(2)
105.0
C2 C3 C4
111.4(3)
111.27
O2
S1
C1
106.4(3)
107.30
C5 C4 C3
110.5(3)
110.94
N1
S1
C1
107.8(3)
107.25
C15 C4 C3
108.4(3)
110.53
C14 O4
C15
118.8(6)
116.59
C15 C4 C5
112.7(3)
111.32
C7
N1
S1
119.7(4)
119.62
C4 C5 C6
112.6(3)
111.53
C2
C1
S1
121.3(4)
119.45
C5 C6 C1
111.2(3)
112.0
C2
C1
C6
119.1(6)
120.22
N1 C7 C1
111.5(3)
113.30
C6
C1
S1
119.6(5)
119.81
C9 C8 C13
119.8(3)
120.71
C1
C2
C3
119.9(6)
119.26
C9 C8 S1
120.6(2)
119.48
C4
C3
C2
121.6(7)
121.18
C10 C11 C14
121.2(4)
120.62
C3
C4
C5
117.8(7)
118.39
C12 C11 C10
117.9(3)
118.39
C3
C4
C17
120.8(7)
120.69
C12 C11 C14
121.0(3)
120.95
C5
C4
C17
121.4(6)
120.89
C11 C12 C13
121.7(3)
121.20
C4
C5
C6
122.2(6)
121.20
C12 C13 C8
119.2(4)
119.2
C5
C6
C1
119.5(6)
119.23
O3 C15 C4
112.6(3)
111.01
N1
C7
C8
112.4(4)
111.57
O4 C15 C4
125.6(4)
125.92
C7
C8
C13
109.6(4)
109.82 13 | P a g e
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O4 C15 O3
121.7(3)
123.05
C9
C8
C7
112.3(4)
112.87
C7 N1 S1
123.7(3)
121.8
C9
C8
C13
111.1(4)
110.14
C15 O3 C16
117.2(3)
115.30
C8
C9
C10
111.7(4)
112.33
N1 S1 C8
108.14(15)
106.89
C11 C10
C9
111.9(4)
111.56
O1 S1 C8
108.02(17)
107.50
C10 C11 C12
109.6(4)
110.74
O1 S1 N1
106.27(14)
104.86
C14 C11 C10
112.2(4)
111.41
C14 C11 C12
110.6(4)
110.27
C13 C12 C11
110.7(4)
111.29
C8 C13 C12
112.2(4)
112.33
O3 C14
O4
122.9(5)
123.79
O3 C14 C11
126.9(5)
125.38
O4 C14 C11
110.2(5)
110.81
C16 C15
112.4(9)
111.34
O4
205 206
3.1
Biological Studies
207
Anti-oxidants serve to protect our body from harms of reactive oxygen species (ROS) like
208
hydrogen peroxide, hydroxyl ion, superoxide and hydroxyl free radical. These oxidants are
209
harmful for our body e.g. converting the enzymes from their active form to non-active one and
210
rupturing of DNA strand [42]. ROS are involved in aging and cell death [43]. In our research
211
work, anti-oxidant potential of carboxylate esters derived from sulfonamide was evaluated by
212
using DPPH scavenging method. Compound (I) (65.27 ± 0.8%: IC50; 173.42 ± 1.2 µg) and (II)
213
(71.05 ± 1.2 %: IC50; 141.18 ± 0.7 µg) showed good anti-oxidant potential which is comparable
214
to gallic acid (77.54 ± 1.4%: IC50; 14.23 ± 0.4µg) a standard anti-oxidant molecule and
215
maximum activity was depicted by (II) as shown in Table 5.
216
Enzymes are the bio-catalyst which acts to control whole body functioning. Any disturbance in
217
an enzyme structure or their over production in body leads to harmful effects in body thus causes
218
major disease. In order to get rid of the diseases caused by enzyme’s extra activity in body, the 14 | P a g e
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219
particular enzyme must be denatured or its activity must be ceased by the use of enzyme
220
inhibiting agents. The synthesized compounds were screened for their inhibitory activity toward
221
enzymes. Acetylcholine esterase (AChE) is the enzyme that is involved in transmission of
222
neurotransmitter acetylcholine in brain and converts the acetylcholine into choline and acetate.
223
Over-functioning of AChE resulted in deficiency of acetylcholine in brain leading to memory
224
loss and hence causes Alzheimer’s disease. In order to cure disease caused by AChE, this
225
enzyme activity must be lowered down or inhibited [44]. Butyrylcholine esterase enzyme
226
(BChE) is also involved in conversion of acetylcholine into choline and acetate and hence the
227
resultant over-activity is related to Alzheimer’s disease [45]. In our research work, esters (I) and
228
(II) have been checked for their enzyme inhibition activity toward both of these enzymes.
229
Compound (I) showed 57.25 ± 1.3 and 53.08 ± 1.1 % inhibition toward AChE and BChE
230
respectively. Whereas (II) gave 62.72 ± 1.4 % inhibition toward AChE while 59.78 ± 0.8 %
231
inhibition toward BChE. α- Chymotrypsin (Protease) enzyme mainly functions in hydrolysis of
232
peptide linkage of proteins. Any over-activity of this enzyme is associated with various diseases
233
in body i.e. joints associated diseases, lung’s diseases and tumor growth [46,47]. α-
234
Chymotrypsin protease enzyme inhibition study was also part of our research work. Synthesized
235
compounds were applied for their inhibition effects against this enzyme. Results showed that
236
synthesized compounds (I) and (II) have 72.56 ± 0.9 and 69.47 ± 1.5% inhibition potential
237
respectively (Table 5).
238
In current research task, the synthesized compounds were also evaluated for their anti-bacterial
239
potential against nine bacterial strains. Both compounds were active against H. halophila, E. coli
240
and S. aureus and their activities were near to standard drugs. However, in remaining were
241
remained inactive and against both fungal strains, synthesized compounds exhibited no activity
242
as shown in Table 6.
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Table 5: Antioxidant and enzyme inhibition potential of I and II
244
Sr #
Sample
DPPH
Enzyme inhibition AChE
*%age
245
**IC
50
*%age
BChE
**IC
50
*%age
Protease
**IC
50
*%age
**IC
50
1
I
65.27 ± 0.8
173.42 ± 1.2
57.25 ± 1.3
183.27 ± 0.7
53.08 ± 1.1
196.13 ± 1.4
72.56 ± 0.9
102.72 ± 1.5
2
II
71.05 ± 1.2
141.18 ± 0.7
62.72 ± 1.4
125.49 ± 1.3
59.78 ± 0.8
178.08 ± 1.1
69.47 ± 1.5
137.53 ± 1.3
3
GA
77.54 ± 1.4
14.23 ± 0.4
-
-
-
-
-
-
4
PMSF
-
-
-
-
-
85.06 ± 0.7
* 100 µL(5 mg/mL)
-
** µg
37.41 ± 0.5
GA; Gallic acid PMSF; standard
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Table 6: Antimicrobial activity of I and II
247
Zone of Inhibition (mm)
Sample A
B
C
D
E
F
G
H
I
J
K
I
5.8 ± 0.8
NIL
NIL
NIL
12.5 ± 1.1
NIL
11.2 ± 0.7
13.7 ± 0.6
NIL
NIL
NIL
II
6.5 ± 1.0
NIL
NIL
NIL
NIL
NIL
15.7 ± 0.5
9.1 ± 0.8
NIL
NIL
NIL
Kanamycin
NIL
NIL
NIL
NIL
NIL
NIL
20.4 ± 0.9
19.3 ± 1.2
NIL
-
-
Ampicillin
26.4 ± 1.4
25.2 ± 1.0
31.5 ± 1.3
50.2 ± 1.7
45.5 ± 0.9
45.3 ± 1.2
26.1 ± 0.8
NIL
30.5 ± 1.1
-
-
Streptomycin
24.8 ± 1.7
24.1 ± 1.1
NIL
35.7 ± 1.3
15.6 ± 0.7
15.2 ± 1.0
25.8 ± 0.9
20.4 ± 1.1
25.7 ± 0.8
-
-
-
-
-
-
-
-
-
-
30.1 ± 1.5
28.4 ± 0.9
Fungizone
-
248 249 A; H. halophila: B; H. salina: C; S. sonnei: D; B. subtilis: E; C. salexigens: F; C. israelensis: G; E. coli: H; S. aureus: I; K. pneumoniae: J; A. niger: K; A. alternata 250 251
Density functional theory calculations have been performed not only to compare the theoretical
252
data with the experimental but also to gain insight into the packing and interaction energies of
253
molecules. The optimized geometries of compounds (I) and (II) are shown in Figure 6 whereas
254
the calculated geometric parameters are compared to the experimental ones in Table 3 and 4.
255
Compound (I) and (II) are structurally very similar, differing only in the ester part. Compound
256
(I) is a methoxy ester whereas compound (II) is an ethoxy ester. The rest of the structures are
257
identical therefore, their geometric parameters are also comparable. Both compounds contain a
258
sulfonamide and an ester functionality each. The calculated S=O bond length (for both S=O
259
bonds) is 1.464 Å for compounds (I) and (II) whereas the experimental S=O bond lengths differ
260
not only between the molecules but also for two S=O bonds in a molecule. The experimental
261
S=O bond lengths in compound (I) are 1.430 and 1.438 Å whereas the similar bond lengths in
262
compound (II) are 1.430 and 1.442 Å. The experimental and calculated C-S bond lengths in
263
compound (I) are 1.763 and 1.797 Å, respectively whereas the corresponding bond lengths in
264
compound (II) are 1.766 and 1.798 A, respectively. The calculated geometric parameters, in
265
general, show good agreement with the experimental geometric parameters. However, the 17 | P a g e
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maximum deviation in the bond lengths is observed for S-N bond lengths where the calculated
267
value for compound (I) (1.678 Å) is somewhat overestimated than the experimental 1.593 Å.
268
The calculated geometric parameters of the ester moiety also agree with the experimental ones.
269
For example, the calculated C=O bond length is 1.212 Å compared to 1.205 Å for the X-ray
270
structure. The C=O bond length of compound (II) shows even better corroboration with the
271
experiment (compare 1.192 and 1.213 for experimental and theoretical, respectively). The
272
efficiency of the theoretical methods for geometric parameters is presented here through root
273
mean square deviations (RMSD). The RMSD for bond lengths for compound (I) and (II) are
274
0.025 and 0.042.
275
276 277
Figure 6: Comparison of the optimized (right) and X-ray geometries (left) of compound 1
278
(top) and 2 (bottom)
279
Bond angles are also compared between the calculated and the X-ray structure. The B3LYP
280
functional performed quite good here as well. Most of the calculated bond angles were within 1
281
degree to the experimental values except a few where the deviation exceeds more than a degree.
282
The maximum deviation of 2.13 degrees in bond angle in compound (I) is observed for C15-C4-
283
C3, an angle which describes the orientation of the ester moiety with respect to the benzene ring.
284
For compound (II), a couple of bond angles deviate more than two degrees; O1-S1-O2 and C14-
285
O4-C15. The former bond angle is present within a sulfonamide group whereas the latter angle
286
represents the orientation of the ethoxy group with respect to carbonyl.
287
3.2
Packing behavior 18 | P a g e
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288
Next, the packing of both compounds in X-ray crystal was considered. Theoretical calculations
289
have been performed for the dimers of compound (I) and (II) and the interaction energies are
290
calculated. For this purpose, input structures were taken from the X-ray geometry. Analysis of
291
the results in Figure 7 reveals that the interaction sites are different for both compounds. In
292
compound (I), the sulfonamide group is in interaction with the protons of cyclohexane moiety.
293
On the other hand, in compound (II), the sulfonamide interacts with the hydrogen atoms of the
294
ethoxy chain. The difference in the interaction is also reflected in the interaction energies.
295
The calculated interaction energies between two molecules in (I) and (II) are 3.18 and 5.30 kcal
296
mol-1. For the packing of third molecule, compound (II) has different behavior than that of
297
compound (I). For compound (I), the nature of interaction is the same as that of dimer. But, for
298
compound (II), the third molecule orients itself in a different way (Figure 8) where aromatic ring
299
interacts with the sulfonamide group. The strength of this additional interaction is estimated
300
about 2.69 kcal mol-1.
301 302
Figure 7: Illustration of the optimized geometries of dimeric (I) and (II), calculated at
303
B3LYP/6-31G(d,p)
304
19 | P a g e
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305 306
Figure 8: Illustration of the packing of compound (II) in the optimized geometry, calculated at
307
B3LYP/6-31G(d,p)
308
309
HOMO
310
LUMO
311
Figure 9. Illustration of HOMOs and LUMOs of compounds (I) (top) and (II) (bottom),
312
calculated at B3LYP/6-31G(d,p)
313
3.3
314
The orbitals of compounds (I) and (II) are also analyzed to gain insight into the distribution of
315
densities in the frontier molecular orbitals (Figure 9). Both compounds show similar distribution
316
of densities in their HOMOs and LUMOs. The HOMOs are mainly localized on the nitrogen
317
atoms of the sulfonamide with some density on the aromatic ring of the sulfonamide whereas the
HOMO-LUMO Study
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318
LUMOs are mainly centered on the aromatic ring. The HOMO-LUMO gaps for compounds (I)
319
and (II) are 5.96 and 5.97 eV. The HOMO-LUMO gaps for both compounds are quite high
320
which indicate their kinetic stability. Since both structures differe only in the aliphatic chain
321
therefore, any significant different in the HOMO-LUMO gaps are not expected.
322
Conclusion
323
Sulfonamide’s carboxylate esters (I) and (II) were synthesized successfully by reacting alcohol
324
(ethanol and methanol) and sulfonamide ligand in acid catalyzed medium. Structures of
325
synthesized compounds were elucidated by using FTIR and single crystal X-ray crystallography.
326
Furthermore, density functional theory (DFT) was done through Gaussian software which also
327
supported the experimental crystallographic data. Both (I) and (II) were screened for their
328
biological potential as enzyme inhibition, antioxidant, antibacterial and antifungal agents. (I) and
329
(II) exhibited appreciable antioxidant and enzyme inhibition potential. They also showed
330
moderate behavior toward anti-bacterial and no activity against fungal strains.
331 332 333 334
ACKNOWLEDGMENT
335
The help of Higher Education Commission is acknowledged for funding this study under the
336
Project No. 20-2549/NRPU/R&D/HEC/12.
337
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1.
25 | P a g e
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Highlights Two ester were synthesized and characterized through XRD analysis DFT studies used to compare experimental and theoretical parameters In-Vitro antimicrobial, antioxidant and enzyme inhibition potential were checked in order to explore their biological importance.
Muhammad Danish, Ayesha Bibi, Khola Gilani, Muhammad Asam Raza, Muhammad Ashfaq, Muhammad Nadeem Arshad, Abdullah Mohamed Asiri, Khurshid Ayub PII:
S0022-2860(18)30943-8
DOI:
10.1016/j.molstruc.2018.07.116
Reference:
MOLSTR 25521
To appear in:
Journal of Molecular Structure
Received Date:
01 June 2018
Accepted Date:
31 July 2018
Please cite this article as: Muhammad Danish, Ayesha Bibi, Khola Gilani, Muhammad Asam Raza, Muhammad Ashfaq, Muhammad Nadeem Arshad, Abdullah Mohamed Asiri, Khurshid Ayub, Antiradical, Antimicrobial and Enzyme Inhibition Evaluation of Sulfonamide Derived Esters; Synthesis, X-Ray Analysis and DFT Studies, Journal of Molecular Structure (2018), doi: 10.1016/j. molstruc.2018.07.116
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ACCEPTED MANUSCRIPT
1
Antiradical, Antimicrobial and Enzyme Inhibition Evaluation of Sulfonamide Derived
2
Esters; Synthesis, X-Ray Analysis and DFT Studies
3
Muhammad Danisha*, Ayesha Bibia, Khola Gilania, Muhammad Asam Razaa, Muhammad
4
Ashfaqa, Muhammad Nadeem Arshadb, Abdullah Mohamed Asirib*, Khurshid Ayubc aDepartment
5 6
bChemistry
Department, Faculty of Science, King Abdulaziz University, Jeddah 21589, Saudi Arabia
7 8
of Chemistry, University of Gujrat, Gujrat 50700 Pakistan
cDepartment
of Chemistry, COMSATS Institute of Information Technology, Abbottabad, KPK,
9
Pakistan, 22060
10
Authors for correspondence:[email protected], [email protected]
11 12
Abstract
13
Two carboxylate esters (methyl: (I) and ethyl: (II)) of 4-{(4-methylphenylsulfonamido)-
14
methyl}cyclohexanecarboxylic acid (sulfonamide) were synthesized and characterized by FTIR
15
and X-ray crystallography. DFT studies were conducted in order to optimize the structures using
16
Gaussian software which confirmed the bond angels and bond lengths obtained from single
17
crystal analysis. Both Compounds (I and II) were evaluated for their biological studies viz;
18
antioxidant activity (DPPH ), enzyme inhibition activity (esterase and proteases), antibacterial
19
(Halomonas halophila, Halomonas salina, Shigella sonnei, Bacillus subtilis, Chromohalobacter
20
salexigens, Chromohalobacter israelensis, Staphylococcus aureus, Escherichia coli and
21
Klebsiella pneumoniae) and anti-fungal (Aspergillus niger and Alternaria alternata). Results
22
depicted that II is more active as compared to I in antioxidant and esterases while I is more
23
potent against protease while moderate results were shown by both.
24
Keywords: Antioxidant; DFT; Enzyme Inhibition; Ester;. Sulfonamide. .
25 26 27
1.
Introduction
28
Sulfonamides have been found to show broad pharmacological profile. They are stable in human
29
body and being used for the treatment of various diseases i.e. tumor, diabetes and other major 1|Page
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pathogens. Moreover, they are used in agriculture field as well as insecticides and herbicides.
31
They are less toxic as compared to other drugs and are scalable
32
that minor variation in the structure of sulfonamide gives vast range of applications both
33
qualitatively as well as quantitatively. Sulfonamides have been proved to be wonderful drugs as
34
they serve the humanity meritoriously for health e.g. as antitumor, antibacterial, antifungal and
35
inhibition against lipoxygenase enzyme [4-7]. As β3 adrenergic agonist, they serve for the
36
treatment of obesity and type 2 diabetes [8-10]. The biological potential of the sulfonamides
37
depends to which way, they attach to their respective receptor or enzyme. This aptitude of
38
binding depends upon proton-ligand complex of the sulfonamides [11]. After the discovery of
39
sulfanilamide, so many chemical alteration have been done and evaluated their therapeutic
40
results.
41
following different synthetic schemes. These syntheses have resulted in the finding of new
42
agents with changeable pharmacological properties [12]. Density functional theory (DFT) has
43
long been renowned as a best tool in the understanding of organic complex previous methods
44
used in the past. Detailed analyses on the performance of various DFT methods have been
45
carried out predominantly for the optimized geometry or structure [13]. Keeping in view such
46
therapeutic applications, new esters derived from sulfonamides were synthesized and
47
characterized. Evaluation of these synthesized compounds for their pharmacological profile
48
involving enzyme inhibition, bactericidal, fungicidal and anti-oxidant potential is also part of this
49
research task.
[1-3]. It has been reported
Up-to date greater than 20,000 sulfanilamide derivatives have been synthesized
50 51
2.
Experimental
52
Chemical for this research task were purchased from Alfa Aesar and Merck (UK). Solvents used;
53
Methanol, Ethanol and Dimethyl Sulfoxide of analytical grade were purchased from Merck
54
(UK). Perkin-Elmer System 100 FT-IR spectrophotometer was used for IR spectral data (4000-
55
400 cm-1) while X-ray diffraction analysis was done on Atlas diffractometer.
56
2.1
57
(I) and Ethyl-4-{(4-methylphenylsulfonamido)methyl} cyclohexanecarboxylate (II)
58
10 mL alcohol (methanol and ethanol) was taken in 100 mL round bottom flask and acidified
59
with 1 mL of conc. H2SO4, followed by the addition of 0.5 gram of 4-{(4-
60
methylphenylsulfonamido)methyl}cyclohexanecarboxylic acid. The mixture was refluxed for
Synthesis of Methyl-4-{(4-methylphenylsulfonamido)methyl} cyclohexanecarboxylate
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61
about 6 hours and stirred overnight at room temperature. After stirring it was concentrated at
62
room temperature via slow evaporation until crystalline product obtained. H3C O
CH3OH
S O
NH
H3C
OCH3
(I)
O S O
O
NH OH
H3C
O
O
C2H5OH
S O
NH OC 2 H5
(II)
63
O
64
2.2
Characterization of the Synthesized Esters
65
Both compounds were characterized on the basis of FTIR and single XRD analysis.
66
2.3
67
Quantum chemical calculations were performed with Gaussian 09 (Revision C.01) [14]. The
68
results are visualized with Gauss View 5.0. The geometries of the compounds are optimized
69
without any symmetry constraints using the hybrid functional B3LYP method 6-31G(d,p) basis
70
set [15]. B3LYP method consists of Becke’s three-parameter (B3) hybrid exchange functional in
71
conjunction with the correlation functional of Lee Yang and Parr (LYP) [16,17]. The basis set
72
chosen contains polarization functions on all atoms. The B3LYP method of DFT is quite reliable
73
for the prediction of geometric and electronic properties of neutral and charged species ranging
74
from simple molecular to polymer structures [18-26]. For optimization, the input geometries are
75
taken from the crystal structure (where available) in order to better match with the
76
experimentally obtained structures. Frequency calculations are also performed at the same level
77
in order to confirm these structures as true minima (absence of an imaginary frequency).
78
2.4
Biological Activities
79
2.4.1
Antimicrobial Assay
DFT studies
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Disc diffusion method was used to measure antimicrobial activity of synthesized compounds
81
against nine bacterial strains; Halomonas halophila, Halomonas salina, Shigella sonnei, Bacillus
82
subtilis, Chromohalobacter salexigens, Chromohalobacter israelensis, Staphylococcus aureus,
83
Escherichia coli, Klebsiella pneumoniae and two fungal strains (Alternaria alternata and
84
Aspergillus niger) according to procedure of Shahid et al., (2009) [27]. Prepared the growth
85
medium, autoclaved at 121oC and transferred 30 mL of this solution to the petri dishes. After
86
solidification of medium, corresponding strain was used to seed medium. 20 µL (5 mg/mL)
87
sample solution was loaded on each disc. Kanamycin, ampicillin and streptomycin were used as
88
reference drugs for bacteria while fungivin was used as antifungal drug. The plates were
89
incubated at 37 oC (24 hours) and 25 oC (48 hours) for bacterial and fungal respectively.
90
2.4.2
91
The methodology of Shahwar et al., (2010) was used to measure the anti-oxidant activity by
92
using radical (2-2’-dienyl-1-picrylhydrazyl) [28]. DPPH solution was prepared in methanol with
93
concentration level of 0.0025g/mL. In first step, added 100µL of each of compound’s sample
94
solution into 2mL DPPH solution in test tube and allowed to stand in darkness for 30 minutes.
95
The absorbance of mixture was recorded at 517 nm keeping methanol was used as blank while
96
Gallic acid was used as standard. % age inhibition was calculated using formula given below.
97
% Inhibition
98
2.4.3
99
Esterases inhibitory activity of synthesized compounds against acetyl cholineesterase (AChE)
100
and butyrylcholine esterase was determined by method of Ellman et al., (1961) along some
101
modifications [29]. 100 μL test compound (5 mg/mL) was mixed with 100 μL enzyme (AChE
102
and BChE) and incubate at 37 °C for 10 minutes. After incubation 0.5 mL buffer (50 mM), 50
103
μL DTNB followed by addition of 50 μL substrate acetylthiocholine iodide and
104
butyrylthiocholine iodide for AChE and BChE respectively. After 30 minutes of incubation at 37
105
°C, the absorbance was measured at 410 nm using UV/VIS spectrophotometer. All experiments
106
were carried out with their respective controls in triplicate. The %age inhibition was calculated
107 108
by the formula mentioned in antioxidant assay.
109
2.4.4
Antioxidant Assay
Absorbance (blank) - Absorbance (test) 100 Absorbance (blank)
Esterases Inhibitory Activity
α-Chymotrypsin Protease Assay 4|Page
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Protease inhibition study of compounds was done by using methodology of Raza, et al., (2013)
111
with minor modifications [30]. In first step, added 100 µL of test sample as well as enzyme,
112
shaked and waited for 10 minutes. 0.5 mL of tris-buffer was added in this solution mixture
113
followed by addition of substrate. Incubation of mixture was done at 37 oC for 30 minutes.
114
Added 0.5 mL distilled water in this solution and recorded the absorbance at 410 nm with UV-
115
VIS spectrophotometer. The %age inhibition was calculated by the formula mentioned in
116
antioxidant assay.
117
3.
118
The sulfonamide was reacted in acidic medium with methanol (I) and ethanol (II) on stirring
119
which resulted white precipitates. The products (I and II) were crystallized in ethanol and
120
characterized with FT-IR and single crystal XRD techniques. In infrared spectra of compounds
121
(I) and (II), the disappearance of broad peak around 3000 cm-1 indicated the deprotonation of
122
acid and formation of ester. Both esters showed the sharper peak in range of 3226 cm-1 (I) to
123
3298 cm-1 (II) indicating the presence of NH group [31]. CH of aliphatic group showed the peak
124
in range of 2922 cm-1 (I) to 2931cm-1 (II). SO2 group gave sharp peaks of the asymmetric and
125
symmetric stretching frequencies in range of 1314 - 1315 cm-1 and 1140 -1146 cm-1 respectively.
126
The stretching frequencies for carboxylate group (COO) were given in the range of 1718 cm-1 (I)
127
to 1720 cm-1 (II) for both compounds showing the confirmation of esters moiety in compounds
128
[32].
Result and Discussion
129
The information about the spatial arrangements of molecules (I and II) in the unit cell is
130
very important for their further physico-chemical properties. Samples of crystallized material
131
were screened out under microscope and glued over a glass fiber tip immersed in a wax on
132
copper rod with magnetic base. This holder was mounted on Agilent Super Nova (Dual source)
133
Agilent Technologies Diffractometer, equipped with graphite-monochromatic Cu/Mo Kα
134
radiation for data collection. The data collection was accomplished using CrysAlisPro software
135
at 296 K under the Mo Kα radiation [33]. The structure solution was performed using SHELXS–
136
97 and refined by full–matrix least–squares methods on F2 using SHELXL–97, in-built with
137
WinGX [34,35]. All non–hydrogen atoms were refined anisotropically by full–matrix least
138
squares methods [34]. Figures were drawn using PLATON and ORTEP-3 [36,37].
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All the hydrogen atoms attached to the aromatic carbon atoms were positioned geometrically and
140
treated as riding atoms with C–H = 0.93 Å and Uiso(H) = 1.2 Ueq(C) carbon atoms. The N-H =
141
0.85(1) Å, hydrogen atom was located with difference fourier map and refined using the DFIX
142
restraint with Uiso (H) = 1.2 Ueq(O). The methyl and methylene hydrogen atoms were also
143
positioned geometrically with C–H = 0.96 Å and Uiso(H) = 1.5 Ueq(C) for methyl group and C–
144
H = 0.97 Å and Uiso(H) = 1.2 Ueq(C) for methylene hydrogen atoms. The Van der Waals’
145
interactions among the molecules produce extra stability of crystal structures. The compound (I)
146
was crystallized with the emphasis to know internal geometry and Van der Waals’ interaction of
147
the molecules in their crystal structures. The study is in continuation of already reported crystal
148
structures of sulfonamides molecules by our group [38,39]. The presented molecule (Figure 1)
149
was crystallized with monoclinic crystal system and P2 1/n space group Table 1. Hydrogen
150
bonding were shown in Table 2 while selected bond lengths and bond angles are provided in
151
Table 3 and 4 respectively.
152
153 154
Figure 1: ORTEP diagram of molecule I where thermal ellipsoids were drawn at 50%
155
probability level
156 157
The cyclohexane ring adopted the chair shape conformation and the root mean square (r. m. s)
158
deviation for the fitted atoms of this ring is 0.2308 Å. The dihedral angles between the planes of
159
cyclohexane atoms and aromatic ring is 21.55 (1)º which is lesser than its parent molecule 4-{(4-
160
methylbenzenesulfonamido)methyl}cyclohexanecarboxylic acid.23 The puckering parameters for
161
the cyclohexane rings are QT = 0.565 (2) Å, θ = 177.8 (5)°, φ = 188.8 (6)° [40]. Methyl-ester
162
group is twisted with the dihedral angle of 53.20 (1) º with respect to cyclohexane ring. A very 6|Page
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163
beautiful network produced through the intermolecular hydrogen bonding which connects the
164
molecules to form the infinite chains along c-axis [0 0 1] as shown in Figures 2 & 3. Atoms N(1)
165
and C(12) in the molecule situated at (x, y, z) act as hydrogen bond donor via H(1N) and H12, to
166
atoms O(4) and O(1) respectively at (x, y, z-1). Both the interactions produced seventeen
167
membered ring motif R22 [41].
168 169 170 171
Figure 2: Unit Cell Diagram of I, showing intermolecular hydrogen bonding interactions
172
using dashed lines
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173 174
Figure 3: Formation of infinite one-dimensional chains along c-axes through hydrogen
175
bonding
176
The molecule II was crystalized in orthorhombic crystal system and unit cell parameters were a =
177
5.3382(3) Å, b = 9.5791(9) Å, c = 36.078(3) Å, V = 1844.8(3) Å3. The data was collected at T =
178
296.15 K with space group P212121 (no. 19) and Z = 4. The final wR2 was 0.1647 (all data)
179
and R1 was 0.0634 (I > 2\s(I)). In the crystal structure of compound II, the O-S-O angle around
180
the S atom is 120.6(2)º giving rise to formation of distorted tetrahedral geometry, where the
181
corner of tetrahedron are being occupied by the C1, N1, O1 and O2 atoms. The dihedral angle
182
between the aromatic ring and plane produced through the fitted atoms of cyclohexane ring is
183
62.086 (2)º. The root mean square (r.m.s) deviation for the cyclohexane ring observed is 0.2318
184
Å and puckering parameters observed are QT = 0.568 (2) Å, θ = 176.99 (5)°, φ = 6.807 (2)°. The
185
ethyl group is disordered over two positions with the site occupancy of 0.73 and 0.27 for major
186
and minor components. Infinite chains observed, produced through the hydrogen bonding
187
interaction between the N-H and SO2 of sulfonamide group. Atoms N1 in the molecule located at
188
(x, y, z) act as hydrogen bond donor via H1N, to atoms O2 at (x-1, y, z).
189
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190
191
Figure 4: Crystal Structure of II
192 193
194
Figure 5: Packing Diagram of II
195 196 197
Table 1: Crystal Data and Structure Refinement of Compound I and II Crystal Data and Structure
I
Refinement Empirical formula Formula weight
C16H23NO4S 325.41
II C17H25NO4S 339.44
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Temperature/K
296(2)
Crystal system
Monoclinic
Space group
P21/n
296.15 orthorhombic P212121
a/Å
7.9687(12)
5.3382(3)
b/Å
25.817(4)
9.5791(9)
c/Å
8.2971(10)
36.078(3)
α/°
90
89.941(7)
β/°
102.959(13)
89.993(6)
γ/°
90
89.995(6)
1663.5(4)
1844.8(3)
Volume/Å3 Z
4
4
ρcalcmg/mm3
1.299
1.222
μ/mm-1
0.212
0.194
F(000)
696.0
728.0
Crystal size/mm3 2θ range for data collection Index ranges Reflections collected Independent reflections Data/restraints/parameters Goodness-of-fit on F2 Final R indexes [I>=2σ (I)]
0.27 × 0.08 × 0.04 5.946 to 57.958° -8 ≤ h ≤ 10, -24 ≤ k ≤ 35, -10 ≤ l ≤ 11 8267 3903[R(int) = 0.0558] 3903/1/202 0.984 R1 = 0.0694, wR2 =
0.420 × 0.270 × 0.210 6.208 to 59.014° -5 ≤ h ≤ 7, -13 ≤ k ≤ 9, 45 ≤ l ≤ 48 9718 4390[R(int) = 0.0472] 4390/0/213 1.019 R1 = 0.0634, wR2 = 10 | P a g e
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0.1351 Final R indexes [all data]
0.1249
R1 = 0.1491, wR2 =
R1 = 0.1492, wR2 =
0.1770
Largest diff. peak/hole / e Å-3
0.1647 0.22/-0.23
0.18/-0.26
Flack parameter
0.77(18)
198
Table 2: Hydrogen Bonds for Compound I
199
D
A
d(D-H)/Å
C12
H12 O11
0.93
2.58
3.447(4)
156.2
N1
H1N O41
0.858(10)
2.098(19)
2.878(4)
151(3)
1+X,
H
d(H-A)/Å
d(D-A)/Å
D-H-A/°
+Y, -1+Z
200
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Table 3: Bond Lengths of synthesized compounds
202
I Atoms
II
Experimental
Theoretical
Atoms
Length/Å
Experimental
Theoretical
Length/Å 1.539
S1
O1
1.430(4)
1.464
1.525(4)
1.537
S1
O2
1.442(4)
1.464
C7
1.526(4)
1.535
S1
N1
1.617(4)
1.681
C2
C3
1.521(4)
1.535
S1
C1
1.766(6)
1.798
C3
C4
1.538(4)
1.535
O3
C14
1.192(6)
1.213
C4
C5
1.513(5)
1.548
O4
C14
1.323(6)
1.354
C4
C15
1.500(4)
1.518
O4
C15
1.467(7)
1.449
C5
C6
1.524(4)
1.534
N1
C7
1.473(6)
1.468
C7
N1
1.467(4)
1.474
C1
C2
1.373(8)
1.395
C8
C9
1.384(5)
1.397
C1
C6
1.393(7)
1.397
C8
C13
1.388(4)
1.395
C2
C3
1.398(9)
1.394
C8
S1
1.763(3)
1.797
C3
C4
1.367(9)
1.401
C9
C10
1.371(5)
1.391
C4
C5
1.374(9)
1.403
C10 C11
1.392(5)
1.403
C4
C17
1.517(9)
1.509
C11 C12
1.379(5)
1.400
C5
C6
1.379(8)
1.392
C11 C14
1.515(5)
1.509
C7
C8
1.523(6)
1.535
C12 C13
1.387(4)
1.394
C8
C9
1.516(6)
1.540
C15 O3
1.329(4)
1.355
C8
C13
1.528(6)
1.540
C15 O4
1.205(4)
1.212
C9
C10
1.524(6)
1.533
C16 O3
1.450(4)
1.436
C10
C11
1.520(6)
1.534
N1
S1
1.593(3)
1.678
C11
C12
1.532(7)
1.547
O1
S1
1.430(2)
1.464
C11
C14
1.507(6)
1.520
C1
C2
C1
C6
C1
1.517(5)
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O2
S1
1.464
1.438(3)
C12
C13
1.528(6)
1.534
C15
C16
1.347(13)
1.520
203
Table 4: Bond Angles of synthesized compounds
204
I Atom
II
Experimental Theoretical
Experimental Theoretical
Atom
Angle/˚
Angle/˚
C2 C1 C6
109.8(3)
110.36
O1
S1
O2
120.6(3)
122.81
C2 C1 C7
112.1(3)
112.15
O1
S1
N1
106.4(3)
106.43
C6 C1 C7
112.1(3)
110.40
O1
S1
C1
108.3(2)
107.19
C1 C2 C3
111.9(3)
111.87
O2
S1
N1
106.9(2)
105.0
C2 C3 C4
111.4(3)
111.27
O2
S1
C1
106.4(3)
107.30
C5 C4 C3
110.5(3)
110.94
N1
S1
C1
107.8(3)
107.25
C15 C4 C3
108.4(3)
110.53
C14 O4
C15
118.8(6)
116.59
C15 C4 C5
112.7(3)
111.32
C7
N1
S1
119.7(4)
119.62
C4 C5 C6
112.6(3)
111.53
C2
C1
S1
121.3(4)
119.45
C5 C6 C1
111.2(3)
112.0
C2
C1
C6
119.1(6)
120.22
N1 C7 C1
111.5(3)
113.30
C6
C1
S1
119.6(5)
119.81
C9 C8 C13
119.8(3)
120.71
C1
C2
C3
119.9(6)
119.26
C9 C8 S1
120.6(2)
119.48
C4
C3
C2
121.6(7)
121.18
C10 C11 C14
121.2(4)
120.62
C3
C4
C5
117.8(7)
118.39
C12 C11 C10
117.9(3)
118.39
C3
C4
C17
120.8(7)
120.69
C12 C11 C14
121.0(3)
120.95
C5
C4
C17
121.4(6)
120.89
C11 C12 C13
121.7(3)
121.20
C4
C5
C6
122.2(6)
121.20
C12 C13 C8
119.2(4)
119.2
C5
C6
C1
119.5(6)
119.23
O3 C15 C4
112.6(3)
111.01
N1
C7
C8
112.4(4)
111.57
O4 C15 C4
125.6(4)
125.92
C7
C8
C13
109.6(4)
109.82 13 | P a g e
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O4 C15 O3
121.7(3)
123.05
C9
C8
C7
112.3(4)
112.87
C7 N1 S1
123.7(3)
121.8
C9
C8
C13
111.1(4)
110.14
C15 O3 C16
117.2(3)
115.30
C8
C9
C10
111.7(4)
112.33
N1 S1 C8
108.14(15)
106.89
C11 C10
C9
111.9(4)
111.56
O1 S1 C8
108.02(17)
107.50
C10 C11 C12
109.6(4)
110.74
O1 S1 N1
106.27(14)
104.86
C14 C11 C10
112.2(4)
111.41
C14 C11 C12
110.6(4)
110.27
C13 C12 C11
110.7(4)
111.29
C8 C13 C12
112.2(4)
112.33
O3 C14
O4
122.9(5)
123.79
O3 C14 C11
126.9(5)
125.38
O4 C14 C11
110.2(5)
110.81
C16 C15
112.4(9)
111.34
O4
205 206
3.1
Biological Studies
207
Anti-oxidants serve to protect our body from harms of reactive oxygen species (ROS) like
208
hydrogen peroxide, hydroxyl ion, superoxide and hydroxyl free radical. These oxidants are
209
harmful for our body e.g. converting the enzymes from their active form to non-active one and
210
rupturing of DNA strand [42]. ROS are involved in aging and cell death [43]. In our research
211
work, anti-oxidant potential of carboxylate esters derived from sulfonamide was evaluated by
212
using DPPH scavenging method. Compound (I) (65.27 ± 0.8%: IC50; 173.42 ± 1.2 µg) and (II)
213
(71.05 ± 1.2 %: IC50; 141.18 ± 0.7 µg) showed good anti-oxidant potential which is comparable
214
to gallic acid (77.54 ± 1.4%: IC50; 14.23 ± 0.4µg) a standard anti-oxidant molecule and
215
maximum activity was depicted by (II) as shown in Table 5.
216
Enzymes are the bio-catalyst which acts to control whole body functioning. Any disturbance in
217
an enzyme structure or their over production in body leads to harmful effects in body thus causes
218
major disease. In order to get rid of the diseases caused by enzyme’s extra activity in body, the 14 | P a g e
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particular enzyme must be denatured or its activity must be ceased by the use of enzyme
220
inhibiting agents. The synthesized compounds were screened for their inhibitory activity toward
221
enzymes. Acetylcholine esterase (AChE) is the enzyme that is involved in transmission of
222
neurotransmitter acetylcholine in brain and converts the acetylcholine into choline and acetate.
223
Over-functioning of AChE resulted in deficiency of acetylcholine in brain leading to memory
224
loss and hence causes Alzheimer’s disease. In order to cure disease caused by AChE, this
225
enzyme activity must be lowered down or inhibited [44]. Butyrylcholine esterase enzyme
226
(BChE) is also involved in conversion of acetylcholine into choline and acetate and hence the
227
resultant over-activity is related to Alzheimer’s disease [45]. In our research work, esters (I) and
228
(II) have been checked for their enzyme inhibition activity toward both of these enzymes.
229
Compound (I) showed 57.25 ± 1.3 and 53.08 ± 1.1 % inhibition toward AChE and BChE
230
respectively. Whereas (II) gave 62.72 ± 1.4 % inhibition toward AChE while 59.78 ± 0.8 %
231
inhibition toward BChE. α- Chymotrypsin (Protease) enzyme mainly functions in hydrolysis of
232
peptide linkage of proteins. Any over-activity of this enzyme is associated with various diseases
233
in body i.e. joints associated diseases, lung’s diseases and tumor growth [46,47]. α-
234
Chymotrypsin protease enzyme inhibition study was also part of our research work. Synthesized
235
compounds were applied for their inhibition effects against this enzyme. Results showed that
236
synthesized compounds (I) and (II) have 72.56 ± 0.9 and 69.47 ± 1.5% inhibition potential
237
respectively (Table 5).
238
In current research task, the synthesized compounds were also evaluated for their anti-bacterial
239
potential against nine bacterial strains. Both compounds were active against H. halophila, E. coli
240
and S. aureus and their activities were near to standard drugs. However, in remaining were
241
remained inactive and against both fungal strains, synthesized compounds exhibited no activity
242
as shown in Table 6.
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Table 5: Antioxidant and enzyme inhibition potential of I and II
244
Sr #
Sample
DPPH
Enzyme inhibition AChE
*%age
245
**IC
50
*%age
BChE
**IC
50
*%age
Protease
**IC
50
*%age
**IC
50
1
I
65.27 ± 0.8
173.42 ± 1.2
57.25 ± 1.3
183.27 ± 0.7
53.08 ± 1.1
196.13 ± 1.4
72.56 ± 0.9
102.72 ± 1.5
2
II
71.05 ± 1.2
141.18 ± 0.7
62.72 ± 1.4
125.49 ± 1.3
59.78 ± 0.8
178.08 ± 1.1
69.47 ± 1.5
137.53 ± 1.3
3
GA
77.54 ± 1.4
14.23 ± 0.4
-
-
-
-
-
-
4
PMSF
-
-
-
-
-
85.06 ± 0.7
* 100 µL(5 mg/mL)
-
** µg
37.41 ± 0.5
GA; Gallic acid PMSF; standard
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Table 6: Antimicrobial activity of I and II
247
Zone of Inhibition (mm)
Sample A
B
C
D
E
F
G
H
I
J
K
I
5.8 ± 0.8
NIL
NIL
NIL
12.5 ± 1.1
NIL
11.2 ± 0.7
13.7 ± 0.6
NIL
NIL
NIL
II
6.5 ± 1.0
NIL
NIL
NIL
NIL
NIL
15.7 ± 0.5
9.1 ± 0.8
NIL
NIL
NIL
Kanamycin
NIL
NIL
NIL
NIL
NIL
NIL
20.4 ± 0.9
19.3 ± 1.2
NIL
-
-
Ampicillin
26.4 ± 1.4
25.2 ± 1.0
31.5 ± 1.3
50.2 ± 1.7
45.5 ± 0.9
45.3 ± 1.2
26.1 ± 0.8
NIL
30.5 ± 1.1
-
-
Streptomycin
24.8 ± 1.7
24.1 ± 1.1
NIL
35.7 ± 1.3
15.6 ± 0.7
15.2 ± 1.0
25.8 ± 0.9
20.4 ± 1.1
25.7 ± 0.8
-
-
-
-
-
-
-
-
-
-
30.1 ± 1.5
28.4 ± 0.9
Fungizone
-
248 249 A; H. halophila: B; H. salina: C; S. sonnei: D; B. subtilis: E; C. salexigens: F; C. israelensis: G; E. coli: H; S. aureus: I; K. pneumoniae: J; A. niger: K; A. alternata 250 251
Density functional theory calculations have been performed not only to compare the theoretical
252
data with the experimental but also to gain insight into the packing and interaction energies of
253
molecules. The optimized geometries of compounds (I) and (II) are shown in Figure 6 whereas
254
the calculated geometric parameters are compared to the experimental ones in Table 3 and 4.
255
Compound (I) and (II) are structurally very similar, differing only in the ester part. Compound
256
(I) is a methoxy ester whereas compound (II) is an ethoxy ester. The rest of the structures are
257
identical therefore, their geometric parameters are also comparable. Both compounds contain a
258
sulfonamide and an ester functionality each. The calculated S=O bond length (for both S=O
259
bonds) is 1.464 Å for compounds (I) and (II) whereas the experimental S=O bond lengths differ
260
not only between the molecules but also for two S=O bonds in a molecule. The experimental
261
S=O bond lengths in compound (I) are 1.430 and 1.438 Å whereas the similar bond lengths in
262
compound (II) are 1.430 and 1.442 Å. The experimental and calculated C-S bond lengths in
263
compound (I) are 1.763 and 1.797 Å, respectively whereas the corresponding bond lengths in
264
compound (II) are 1.766 and 1.798 A, respectively. The calculated geometric parameters, in
265
general, show good agreement with the experimental geometric parameters. However, the 17 | P a g e
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266
maximum deviation in the bond lengths is observed for S-N bond lengths where the calculated
267
value for compound (I) (1.678 Å) is somewhat overestimated than the experimental 1.593 Å.
268
The calculated geometric parameters of the ester moiety also agree with the experimental ones.
269
For example, the calculated C=O bond length is 1.212 Å compared to 1.205 Å for the X-ray
270
structure. The C=O bond length of compound (II) shows even better corroboration with the
271
experiment (compare 1.192 and 1.213 for experimental and theoretical, respectively). The
272
efficiency of the theoretical methods for geometric parameters is presented here through root
273
mean square deviations (RMSD). The RMSD for bond lengths for compound (I) and (II) are
274
0.025 and 0.042.
275
276 277
Figure 6: Comparison of the optimized (right) and X-ray geometries (left) of compound 1
278
(top) and 2 (bottom)
279
Bond angles are also compared between the calculated and the X-ray structure. The B3LYP
280
functional performed quite good here as well. Most of the calculated bond angles were within 1
281
degree to the experimental values except a few where the deviation exceeds more than a degree.
282
The maximum deviation of 2.13 degrees in bond angle in compound (I) is observed for C15-C4-
283
C3, an angle which describes the orientation of the ester moiety with respect to the benzene ring.
284
For compound (II), a couple of bond angles deviate more than two degrees; O1-S1-O2 and C14-
285
O4-C15. The former bond angle is present within a sulfonamide group whereas the latter angle
286
represents the orientation of the ethoxy group with respect to carbonyl.
287
3.2
Packing behavior 18 | P a g e
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288
Next, the packing of both compounds in X-ray crystal was considered. Theoretical calculations
289
have been performed for the dimers of compound (I) and (II) and the interaction energies are
290
calculated. For this purpose, input structures were taken from the X-ray geometry. Analysis of
291
the results in Figure 7 reveals that the interaction sites are different for both compounds. In
292
compound (I), the sulfonamide group is in interaction with the protons of cyclohexane moiety.
293
On the other hand, in compound (II), the sulfonamide interacts with the hydrogen atoms of the
294
ethoxy chain. The difference in the interaction is also reflected in the interaction energies.
295
The calculated interaction energies between two molecules in (I) and (II) are 3.18 and 5.30 kcal
296
mol-1. For the packing of third molecule, compound (II) has different behavior than that of
297
compound (I). For compound (I), the nature of interaction is the same as that of dimer. But, for
298
compound (II), the third molecule orients itself in a different way (Figure 8) where aromatic ring
299
interacts with the sulfonamide group. The strength of this additional interaction is estimated
300
about 2.69 kcal mol-1.
301 302
Figure 7: Illustration of the optimized geometries of dimeric (I) and (II), calculated at
303
B3LYP/6-31G(d,p)
304
19 | P a g e
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305 306
Figure 8: Illustration of the packing of compound (II) in the optimized geometry, calculated at
307
B3LYP/6-31G(d,p)
308
309
HOMO
310
LUMO
311
Figure 9. Illustration of HOMOs and LUMOs of compounds (I) (top) and (II) (bottom),
312
calculated at B3LYP/6-31G(d,p)
313
3.3
314
The orbitals of compounds (I) and (II) are also analyzed to gain insight into the distribution of
315
densities in the frontier molecular orbitals (Figure 9). Both compounds show similar distribution
316
of densities in their HOMOs and LUMOs. The HOMOs are mainly localized on the nitrogen
317
atoms of the sulfonamide with some density on the aromatic ring of the sulfonamide whereas the
HOMO-LUMO Study
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318
LUMOs are mainly centered on the aromatic ring. The HOMO-LUMO gaps for compounds (I)
319
and (II) are 5.96 and 5.97 eV. The HOMO-LUMO gaps for both compounds are quite high
320
which indicate their kinetic stability. Since both structures differe only in the aliphatic chain
321
therefore, any significant different in the HOMO-LUMO gaps are not expected.
322
Conclusion
323
Sulfonamide’s carboxylate esters (I) and (II) were synthesized successfully by reacting alcohol
324
(ethanol and methanol) and sulfonamide ligand in acid catalyzed medium. Structures of
325
synthesized compounds were elucidated by using FTIR and single crystal X-ray crystallography.
326
Furthermore, density functional theory (DFT) was done through Gaussian software which also
327
supported the experimental crystallographic data. Both (I) and (II) were screened for their
328
biological potential as enzyme inhibition, antioxidant, antibacterial and antifungal agents. (I) and
329
(II) exhibited appreciable antioxidant and enzyme inhibition potential. They also showed
330
moderate behavior toward anti-bacterial and no activity against fungal strains.
331 332 333 334
ACKNOWLEDGMENT
335
The help of Higher Education Commission is acknowledged for funding this study under the
336
Project No. 20-2549/NRPU/R&D/HEC/12.
337
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1.
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Highlights Two ester were synthesized and characterized through XRD analysis DFT studies used to compare experimental and theoretical parameters In-Vitro antimicrobial, antioxidant and enzyme inhibition potential were checked in order to explore their biological importance.