سلطان کھاروی دیاںکافیاں
کجھ و دواناں دے وچار نیں کہ کافی عربی زبان دا لفظ اے جیدے معنی نیں مکمل ، پورا یا کافی ہونا۔ کیوں جے قرآن مجید وچ ربی فرمان اے۔
’’ کفیٰ باللہ شہیدا اللہ دی گواہی کافی اے ‘‘ (۱)
’’ کفیٰ باللہ وکیلا اللہ کارساز کافی اے ‘‘(۲)
’’قرآن حکیم وچ ایہہ لفظ کافی تے مکمل دے معنی وچ استعمال ہویا اے۔ ایس لئی شاعری دی اجہی صنف نوں کافی آکھیا گیا ہے۔ جہدے وچ اک مکمل مضمون اک مکمل خیال یاں اک مکمل جذبے دا اظہار کیتا گیا سی۔ شاعری دی ایس صنف نوں پڑھ کے یاںسن کے ہور کسے صنف یاں شاعری دے مطالعے یاں سنن دی لوڑ نہیں رہندی ۔ کیوں جے ایہدے راہیں بیان ہون والا مضمون یاں خیال ، ادبی ذوق ، روحانی لوڑاں تھوڑاں تے وجدان دی مکمل حد تک تسکین کر دیندا اے۔ ایسے پاروں شاعری دی ایس صنف نوں کافی آکھیا گیا اے۔‘‘(۳)
کافی تے سنگیت دا آپسی گوہڑا سمبندھ ہے ۔ کافی وچ سنگیت پکھ اگھڑواں ہوندا اے۔ ایس لئی سنگیت توں بنا ں کافی مکمل نہیں ۔جے ایہہ آکھیا جاوے کہ شاہ حسین نے کافی تے سنگیت نوں لازم و ملزوم بنا دتا اے تاں کجھغلط وی نہ ہووے گا۔ اونہاں اپنیاں کافیاں بارے واضح شبداں وچ لکھ دتا، پئی ایہہ کافی فلاں راگ یاں راگنی وچ گائی جاوے مثال دے طور تے اوہناں نے اپنی ایس کافی نوں راگ جے جے ونتی وچ گاون دی ہدایت کیتی اے۔
متراں دی مجمانی خاطر دل دا لہو چھانی دا
کڈھ کلیجہ کیتم بیرے سو بھی...
It is evident from the teaching of Quran & Sunna, Allah SWT accepts the repentance of His servants. The concept of repentance is according to synthesis of human nature. As a matter of fact, the commission of sins is deep rooted into the human nature and except the messengers of Allah SWT, who are by their nature immaculate and impeccable, all the human beings commit the sins in one form or the other. However, the countless mercy of Allah SWT is showered upon the servants in the shape of “tauba” or repentance. The concept of repentance infuses a new life into the sinful soul of human being. The tauba or seeking forgiveness of Allah SWT revitalizes the enthusiasm of worship in the Muslim. The concept of the acceptance of tauba provide the peace of mind, consolation and satisfaction of heart to the believers. It enables him to reconnect himself to his Lord. Once a person realizes the forgiveness of Allah SWT, he feels a unique tranquility in his heart. This paper will investigate the multiple verses of Quran and Prophetic Sunna concerning the tauba and istaghfar, and how it helps us to attain the peace of mind and acquire satisfaction of heart.
Biodegradation of organic pollutants such as polycyclic aromatic hydrocarbons using soil microorganisms where they use these compounds as carbon and energy source, is the safe, cheap and environment friendly way. In the present study bacterial samples were isolated from crude oil contaminated soil. A total of 52 isolates were initially screened, fifteen of these isolates were checked for growth on PNR medium containing up to 1200 and 800 ppm, anthracene and pyrene, respectively. Five bacterial isolates were selected on the basis of their best on PAHs growth and identified as Bacillus cereus KWS2, Bacillus cereus KWS4, Bacillus licheniformis DW3, Bacillus licheniformis Sol-10, and Pseudomonas stutzeri 10-1. Biodegradation studies of anthracene were carried out by Bacillus cereus KWS2 at different pH, temperature and incubation time. The optimum pH and temperature were 7 and 30oC respectively, for degradation and growth where 45 % of reduction in anthracene concentration was observed after seven days of incubation. Growth was maximum after 2 days of incubation (12 x 10 7 CFU/mL). Pseudomonas stutzeri 10-1 was also checked for anthracene and naphthalene degradation capability. 33.81 % reduction in naphthalene concentration was observed after one week, while 33.69 and 45.35 % reduction after two and three weeks time, respectively. In case of anthracene, 87.37 % reduction was observed after first week of incubation whereas 92.98 and 95.56 % was observed after two and three weeks, respectively. Resting cell biotransformation studies of naphthalene, phenanthrene and anthracene were carried out by Bacillus cereus KWS2 and KWS4, analyzed by GC/MS. From naphthalene biotransformation four metabolites, 2-naphthol, benzeneacetic acid, benzoic acid and benzaldehyde were detected and identified. From phenanthrene biotransformation, 9-phenanthrenol, 9,10-Dihydro,9,10-dihydroxyphenanthrene, bezeneacetic acid, 4-hydroxy-benzeneacetic acid and 2-hydroxy benzoic acid were detected and identified. Benzenecarboxylic acid, benzeneacetic acid and 4-hydroxy- benzeneacetic acid were detected and identified from anthracene biotransformation by B. cereus KWS2. The detection of both mono and dihydroxylated compounds x suggested that B. cereus strains KWS2 & KWS4 harbor both mono and dioxygenase genes. Biotransformation potential of a selected bacterial isolate, Mycobacterium PY146 for PAHs was studied. Resting and growing cell biotransformation of PAHs including phenanthrene, anthracene and pyrene by Mycobacterium PY146 one metabolite i.e, 1,2-benzenedicarboxylic acid (phthalic acid) from phenanthrene and two metabolites, 1,2-benzenedicarboxylic acid and 9,10-anthracendione from the anthracene biotransformation, where as two metabolites, 1,2-benzenedicarboxylic acid and 1- hydroxypyrene were detected and identified from pyrene biotransformation. While in growing cell biotransformation of phenanthrene, 1,2-benzenedicarboxylic acid and benzeneacetic acid, from anthracene 9,10-anthracenedione, benzenecarboxylic acid, benzeneacetic acid and 1,2-benzenedicarboxylic acid and from pyrene benzenecarboxylic acid, benzeneacetic acid and 1,2-benzenedicarboxylic acid were detected and identified. Biodegradation of PAHs including phenanthrene, anthracene and pyrene were checked in soil by Mycobacterium PY146 without and with yeast extract. After one week of incubation the detectable concentration of PAHs without yeast extract, phenanthrene (98 μg), anthracene (60 μg) and pyrene (56 μg) were decreased to 35, 18 and 27 μg, and after 2 weeks of incubation all of the detectable PAHs were 0.14, 0.45 and 0.19 μg respectively. There was no significant effect of yeast extract on degradation except phenanthrene, which decreased from 98 to 27 μg after one week. Mineralization studies of different 14 C-PAHs (naphthalene, phenanthrene, pyrene and benzo(a)pyrene) were carried out by Bacillus cereus KWS2 and Mycobacterium PY146. In case of naphthalene and phenanthrene mineralization by Bacillus cereus KWS2, no mineralization was observed. Mineralization of phenanthrene, pyrene and benzo(a)pyrene by Mycobacterium PY146 showed that 45.92, 39.89 and 4.82 % of 14 CO 2 was produced and detected in the form of Na 214 CO 3. The mineralization of 14 C pyrene and phenanthrene with the different cell densities from OD 600 0.1 to 0.5 of Mycobacterium PY146 cultures showed that the maximum mineralization of pyrene was observed in the OD 600 0.2 culture, while in the case of xi phenanthrene there is increase in mineralization between the OD 600 0.1 to 0.2 culture. There was subsequent decrease in both pyrene and phenanthrene mineralization as the cell density increases. The expression of pyrene dioxygenase gene (nidAB) from Mycobacterium PY146 was checked in E. coli by cloning the nidAB in pKK223-3 expression vector and then transformed the E. coli. The biotransformation of naphthalene, phenanthrene, anthracene and pyrene was checked using transformed E. coli cells containing nidAB. Neither any hydroxy nor any derivatized metabolite were detected of any PAH after derivatization with N,O-Bis(trimethylsilyl)trifluoroacetamide with 1 %Trimethylechlorosilane (BSTFA). Quantification of nidAB RNA transcripts in E. coli was done by RT-QPCR which revealed an ~ 2- fold increase in RNA transcripts in one sample grown in the presence of IPTG. RNA to DNA ratio of nidAB calculated by RT-QPCR was increased between OD 600 0.1 to 0.4 and then declined at and OD 600 of 0.5. Relation of phenanthrene and pyrene mineralization to RNA/DNA ratio with the OD 600 from 0.1 to 0.5 showed the positive relationship between phenanthrene mineralization and the RNA/ DNA ratio while in case of pyrene only the OD 600 of 0.3 to 0.5 corresponds to the ratio. From the present study, it is concluded that soil is the rich source of microbes having the degradative capability of pollutants like PAHs. Some microbes have the ability to degrade and mineralize the PAHs efficiently while others can only transform but can’t mineralize. The expression and the RNA transcript of pyrene dioxygenase (nidAB) copy number and RNA/DNA ratio correspond to the mineralization of PAHs.