Cellulase constitute the third largest group of enzymes employed in the industry for the processing of food, textile, detergents, paper and pulp and conversion of agricultural biomass into bio fuel and other useful products. The present study therefore was focused on production of cellulases from Trichoderma harzianum for employing in various applications. Trichoderma harzianum after qualitative screening on carboxymethyl cellulose agar and cellulose Azure was utilized for the production of endoglucanase, exoglucanase and β- glucosidase. Mandel`s mineral salt medium was found to be suitable for the production of cellulases in submerged culture at 120rpm. Significant improvements in specific activities of cellulases were recorded in the Mandel’s salt medium supplemented with 3% wheat bran and 0. 06% lactose as an inducer and addition of Tween 80 further facilitated cellulase production. Maximum production of all the enzymes was achieved between 72 -96 hours of fermentation in most of the production parameter notable activities were achieved at 96 hours. The enzyme production was favorable at temperature of 25°C and 30°C with optimum production reported at 30°C with significant specific activities of endoglucanase (137.3U/mg), exoglucanase (80.63 U/mg) and β-glucosidase (106.88 U/mg). pH 5.0 brought significant production of endoglucanase (139.26 U/mg), exoglucanase(90.12 U/mg) and β-glucosidase (109.88U/mg). Purification was carried out on Sephadex G-100, which revealed two distinct peaks of enzyme activity. Lyophilized fractions with 425.7% yield for endoglucanase, 464. 6% exoglucanase and 468% β-glucosidase were subjected to SDS-PAGE for the determination of molecular weights that resulted in separation of protein into five bands of 95KDa, 75 KDa, 65KDa, 60KDa and 20KDa. Characterization of crude and purified cellulases indicated maximum residual activities of crude cellulases between 35-55°C with maximum activities attained at 45°C. The temperature optima of purified cellulases shifted from 45°C to 50°C for endoglucanse and exoglucanase and to 55°C for β-glucosidase. Study of residual activity of crude and purified cellulases in varying pH revealed that the enzymes have a broad pH range both crude and purified fractions were most active at pH5- _______________________________________________________________________________ Production, Purification & Characterization of Cellulases from Trichoderma harzianum in Sub merged Condition & their Applications. 6. 5 with maximum residual activities retained at pH 5.5. Metal ions like Mn2+, Zn2+, Ca2+, Mg2+, K, and Na had stimulatory effect on the activity of crude as well as purified cellulases Fe2+ ion neither inhibited nor had a stimulatory effect. Lead, Hg2+ and Cu2+ had maximum inhibitory effect. Co2+ inhibited endoglucanase and exoglucanase activity while a slight inhibition was reported in case of β-glucosidase. Enzyme activities of purified enzymes were stimulated by mercaptoethanol. SDS and EDTA had a slight inhibitory effect. Crude enzyme were supplemented in a high fiber formulated poultry feed. Seven dietary treatments comprising of four dietary doses of cellulases only, two dietary mixed doses with cellulases and proteases and a dietary dose without enzyme supplementation that was kept as a control were fed to birds over a period o f 43 days. Enzyme supplementation resulted in increase in average weight gain of all the treatments when compared with control. 156g more weight than control group (A) was recorded in group E (16ml cellulase /kg feed) on 43rd day. A decrease in feed conversion ratio was recorded in all the treatment groups that were linear with increasing enzyme doses. With increasing cellulase dose a decrease in viscosity was noted. In vitro maximum viscosity (1.29 cP) was recorded in control group (A) and minimum was in group E (0.712 cP). Similar results were reported for In vivo viscosity studies of digesta from live birds with maximum figure (1. 089 cP) in control group (A) and maximum reduction was attained in group E (0.521). Dry matter digestibility in control group (80.58%) was less than in all treatment groups with maximum reported in group G (91.08%). Deinking of different type of waste paper resulted in increase in color units of all treated pulps over their respective controls. An average of 2% increase in brightness index of all treated pulps was achieved. Image analysis revealed reduction of residual ink (%) in all the enzyme treated hand sheets. The crude enzyme was found to be stable in all five commercial detergents used, with 90% of residual activity retained after 1 hour of incubation at 40 °C in detergent A. More than 40% residual activity was retained in rest of the detergents after one hour. The crude enzyme was active in removing/fading different type of stains and along with detergent the cleaning power was enhanced further. The crude preparation of cellulases was also successful in biostoning of denim bringing out an even faded look of the garment with an additional advantage of negligible back staining.
ذوالفقار علی بھٹو شہید نے صرف چار سال اور بیس دن سیاست جبکہ پانچ سال ،چھ ماہ اور پندرہ دن حکومت کی جس کے بعد پھانسی کی سزا ہوئی ۔تحریک ،قتدار اور اسیری کا یہ کل دورانیہ بارہ سال اور پانچ دن ہے ۔نواز شریف کو سیاست میں تیس برس گزر چکے ہیں ۔مولانا فضل الرحمن کو سینتیسواں سال ہے اور عمران نیازی کو بائیس سال ۔
ذوالفقار علی بھٹو شہید کو پھانسی دینے والے ڈکٹیٹر کو بھی قتدار کے گیارہ سال ایک ماہ اور بارہ دن ملے مگر ان میں سے کوئی بھی ذوالفقار علی بھٹو شہید کا متبادل نہ بن سکا ۔اب یہ بھٹو کا کرشمہ ہے یا بھرپور طاقت اور وقت ملنے کے باوجود متبادل بننے کی کوشش کرنے والے لیڈروں کی نااہلی کہ بھٹو زندہ ہے ۔
دنیا کی تاریخ میں بہت کم ایسے لیڈر ہیں جنہوں نے اتنے گہرے اثرات مرتب کیے ہیں ۔ایسا صرف مذہبی تحریکوں میں ممکن ہوا ہے یا بھٹو نے ممکن کر دکھایا ہے ۔بھٹو ضدی تھا ۔اسے جب تک تسلیم نہیں کیا جائے گا اور وہ اپنی جنگ جیت یگا ۔کہیں لکھ کر رکھ لیں وہ مرنے والا نہیں ۔ذوالفقار علی بھٹو شہید نے کہا تھا کہ آخری قہقہہ عوام کا ہو گا ۔
مجھے لگتا ہے کہ پاکستان کے عوام ادھر وہ قہقہہ لگائیں گے اور ادھر بھٹو آنکھ مار کر مر جائے گا ۔ذوالفقار علی بھٹو شہید صرف پاکستان پیپلز پارٹی کی پراپرٹی نہیں ہے بلکہ یہ پاکستان کی پراپرٹی بھی ہے ۔وہ ہمارا منتخب وزیر اعظم تھا ۔ہمیں دوسرے خطوں سے ہیروز امپورٹ کر نے پڑتے ہیں ۔بھٹو ہمار ا وہ مقامی ہیرو ہے جسے ہم دنیا میں ایکسپورٹ کرتے ہیں ۔
Tujuan dari penelitian ini adalah untuk memahami sejauh mana Implementasi kebijakan pemerintah dalam pencegahan penyebaran Covid19, untuk mengetahui implementasi kebijakan pemerintah terhadap masyarakat dan mengetahui faktor yang mempengaruhi dalam pencegahan penyebaran Covid 19. Penelitian ini dilakukan di Kantor Dinas Kesehatan Kota Padang dan Badan Kesatuan Bangsa dan Politik. Penelitian ini menerapkan teknik analisis kualitatif menggunakan pendekatan deskriptif. Hasil dan kesimpulan dari penelitian ini adalah pemerintah telah menerapkan beberapa kebijakan dalam penanganan covid19 diantaranya melakukan pemberian pelayanan kesehatan masyarakat selama masa pandemi. Peraturan yang telah dibuat harus selalu dipatuhi mengingat faktor penghambat dari implementasi kebijakan ini adalah kesadaran diri terhadap bahaya virus Covid19.
Hepatitis C is a major health problem affecting more than 200 million individuals in World including Pakistan. Current treatment regimen consisting of interferon alpha and ribavirin does not always succeed to eliminate virus completely from the patient’s body. The mechanism how Hepatitis C Virus (HCV) induces interferon resistance is still indefinable. HCV genotype 1a shows greater hindrance to treatment than genotype 3a. One of the mechanisms by which virus evades the antiviral effect of interferon alpha involves that HCV envelope protein 2 (E2) interacts with Protein Kinase (PKR) which is the interferon-inducible protein kinase and which in turn blocks the activity of its target molecule called eukaryotic translation initiation factor 2 alpha (eIF2α). Sequence analysis of Envelope protein reveals it contains a domain homologous to phosphorylation sites of PKR and the translation initiation factor eIF2alpha. This domain is known as protein kinase (PKR) eukaryotic initiation factor 2 alpha (eIF2α) phosphorylation homology domain (PePHD). This domain in HCV genotype 1 strains is reportedly homologous to PKR and its target eIF2α. Thus envelope protein competes for phosphorylation with PKR. By binding to PKR, PePHD inhibits its activity and therefore cause virus to evade antiviral activity of interferon (IFN). In the present study the possible role of phosphorylation in envelope 2 protein for interferon resistance was first investigated in silico and then confirmed invivo. Genes coding for envelope 2 protein were isolated from local HCV isolates and their tertiary structure was predicted. Insilico phosphorylation of tertiary structures revealed that two residues S75 and S277 of envelope 2 gene are surface exposed at cytoplasmic domain and may compete with the phosphorylation of PKR protein. Interferon induced antiviral protein PKR has a role in the HCV treatment as dsRNA activated PKR has the capacity to phosphorylate the serine and threonine of E2 protein and dimerization of viral RNA. E2 gene of HCV genotype 1 has an active role in IFN resistance. E2 protein inhibits and terminates the kinase activity of PKR by blocking it in protein synthesis and cell growth. This brings forward a possible relation of E2 and PKR through a mechanism via which HCV evades the antiviral effect of IFN. A hybrid in-silico and wet laboratory approach of motif prediction, evolutionary and structural analysis has pointed out serine 75 and 277 of the HCV E2 gene as a promising candidate for the serine phosphorylation. It is proposed that Serine phosphorylation of HCV E2 gene has a significant role in interferon resistance. In present study we mutated the two Serineresidues at positions S75 and S277 and their efficacy was checked in respect to interferon resistance. The results of this study suggest that serine residues as predicted have a significant role in interferon resistance, especially S75. It is also suggested that some other factors may be involved along with viral envelope gene 2.