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Home > Petrology of Mansehra Granitic Complex, Hazara Area, Northwestern Himalaya, Pakistan

Petrology of Mansehra Granitic Complex, Hazara Area, Northwestern Himalaya, Pakistan

Thesis Info

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Author

Naeem, Mustansar

Program

PhD

Institute

University of the Punjab

City

Lahore

Province

Punjab

Country

Pakistan

Thesis Completing Year

2012

Thesis Completion Status

Completed

Subject

History & geography

Language

English

Link

http://prr.hec.gov.pk/jspui/bitstream/123456789/2369/1/3001S.pdf

Added

2021-02-17 19:49:13

Modified

2024-03-24 20:25:49

ARI ID

1676724921197

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The Mansehra Granitic Complex (MGC) is mainly comprised of Mansehra Granite (MG), Hakale Granite (HG), microgranitic (MIG) and leucogranitic (LG) bodies along with pegmatites and aplites. Geochemical classification diagrams place these granites in the high calc-alkaline, quartz-rich, peraluminous granitoid field. The Mansehra Granite is a porphyritic and massive body that is locally foliated, whereas the Hakale Granite is sub-porphyritic to non-porphyritic pluton. The Susalgali Granite Gneiss is sheared Mansehra Granite. Harker’s variation diagrams show that MG and HG are derived from magmas of the common non- homogeneous source rock Tanawal Formation through fractional crystallization process in a closed system without considerable contamination. Field relationships, geochemical and mineralogical characteristics of the MGC reveal the peraluminous S-type nature of this Complex. The zircon saturation temperature of MG (749-852 oC), HG (709-779 oC), LG (749-754 oC) and MIG (692-696 oC) is comparable with crystallization temperatures of the peraluminous S-type Lesser Himalayan Indian granites (~670-817 oC). The geochemical characteristics of the MG revealed that the magma was probably generated through biotite dehydration melting of the metasediments of Tanawal Formation at pressure > 5 kbr and temperature > 700 oC, while HG melt was most likely originated at relatively shallower crustal level and lower temperature by muscovite fluid-absent melting of pelites. The occurrence of andalusite in the contact aureole of Mansehra Granite, association of perthitic microcline along negative Nb, Sr and Ti anomalies in spidergrams and higher Rb/Sr ratios in granitic rocks of the MGC may reveal the upper crustal signatures and low pressure shallow emplacement (< 15 km) of these bodies. The leucogranitic bodies associated with the MGC are most likely the products of Na 2 O-rich residual melt of the MG, whereas microgranites may have been derived from boron-rich residual magma of the HG by insurgent boiling and subsequent quenching. In the light of U-Pb zircon systematics of the MGC, a middle Mesoproterozoic to early Neoproterozoic age (ca. 1300-985 Ma) has been proposed for the granite protolith in Hazara area. Whereas, the inherited age components of ca. 985-920, vi880-800 and 690-500 Ma may be interpreted as the ages of post-depositional metamorphic fabric development in the source Tanawal Formation. U-Pb zircon dating of Lesser Himalayan granites also revealed inherited age components at ca. 980 ca. 800 Ma and ca. 700-500 Ma. The age segments of ca. 490 Ma, ca. 475 Ma and ca. 466 Ma (middle to upper Ordovician) represent the intrusive ages of the MG, LG and HG, respectively. The mean age of Mansehra Granite (ca. 480 Ma) is younger than the reported Rb/Sr age of 516±16 Ma (Le Fort et al., 1980). The U-Pb zircon systematics of Mansehra Granite is comparable with the reported Rb/Sr and U-Pb zircon ages of the Himalayan granites and gneisses. Moreover, the depletion of Ba, Sr, Nb and Ti in spidergrams of the MGC allows correlation with the early Paleozoic (500±25 Ma) Lesser Himalayan S-type granites. According to the similarity of mineralogical, geochemical, structural features and U-Pb zircon dating of the MGC (ca. 466-490 Ma) with the peraluminous S-type Himalayan granites, it may be assumed that Mansehra Complex is associated with the Pan African orogeny. However, convincing evidence is lacking. Hence, the genesis of MGC can be better explained by emplacement of Cambro- Ordovician granites along the northern margin of Gondwana.
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حضرت مولاناقاری نیاز احمد مرحوم

حضرت مولانا قاری نیاز احمد مرحوم

قاری نیاز احمد سرکار
حقیقت دے وچ سن اوہ رب دے یار
سوہنا خلق تے سوہنی صورت ہر اک نوں پئی بھاوے
جیہڑا ملدا ہک واری او ول ول ملنے آوے
کرن دعا رب دیوے شفاء سوہنا سائیں کرم فرماوے
غم اندوہ سب دور ہوجاندے جیہڑا ملدا سی ہک وار

بہاول نگر توں ٹامیوالی مرشد نے بھجوایا
ساوی مسجد ڈیرا لاء کے دین اسلام پھیلایا
قرآن شریف تے فقہ فقر دا نالے درس حدیث پڑھایا
وعظ کلام انہاں دا سن کے توبہ کردے اوگن ہار

ایڈا چرچا شہرت ہوئی ہر کوئی آپ نوں بھالے
دین اسلام دے آپ حضور نے ہر جا دیوے بالے
کفر و شرک مٹایا آپ نے ہر جا تھئے اجالے
دینی جذبہ ویکھ کے لوگ ہو گئے تابعدار

سادے کپڑے سادہ کھانا خوش اخلاق بتہرے
جس تے نظر کرم دی پاندے کردے دور اندھیرے
واہ نصیب انہاں دا جینہاں کیتے درشن تیرے
یاد تہاڈی بڑا ستاندی دل روندا زار و نزار

ظاہر باطن پاک انہاں دا رزق حلال کماندے
آل اولاد تے آن والا نوں رزق حلال کھواندے
ہر اک نوں تاکید سی کردے جو در سرکار تے آندے
نہ اوہ محفل نہ اوہ رونق کتھے ٹر گئے ہو سرکار

قادری سائیںؔ یاد انہاں دی دل وچ ورمی بہہ گئی
ایڈا درد وچھوڑے والا کیویں ایہہ جندڑی سہہ گئی
رب راضی تے ہر کوئی راضی جگ وچ گل انہاں دی رہ گئی
پر وچھڑے یار نہ بھلدے بھاویں گزرن سال ہزار

An Evaluation of the 2020 Change to the Saudi Emergency Residency Program Assessment

Background Several changes have been made to the assessment component of Saudi residency training programs. Among those is the implementation of three examinations over the course of the year. Aim We aimed to explore the emergency residents’ perspective on the change in the number of examinations, and the impact of such changes in terms of time management, knowledge gain, and social life. Methods This cross-sectional study was carried out from September to October 2022, using an electronic survey targeting emergency board trainees. Results One hundred and nine emergency residents enrolled, of whom 64.2% were male. The majority, 45%, were from the central province. Junior-level residents (R1) represented 26.6% of the sample, while R2 (second year) comprised 18.3%, R3 (third year) comprised 38.5%, and 16.5% were senior (R4) level. More than half of the participants, 56 % (n=61), did not support the change from one to three examinations and believed that it had a negative influence on knowledge gain and clinical skills. The influence of the change on time management stands out as a negative impact, in addition to its impact on social life and annual leave arrangements. Conclusions The support for three examinations throughout the year was low; a contributing factor to this may be the sudden changes effected by those tests on training and time management. A re-evaluation of testing culture and involving residents in decision-making might generate acceptance.

Identification of Nanoviruses in Banana from Pakistan and Possible Control Through Rnai

Banana Bunchy Top Virus (BBTV) is a member of genus Babuvirus of the family Nanoviridae, ssDNA virus transmitted by Pentalonia nigronervosa. Family Nanoviridae is divided into two genera: Nanovirus and Babuvirus. Nanovirus includes FBNYV, MDV, SCSV, while the genus Babuvirus include BBTV. In Pakistan, banana production is under severe loss due to BBTV. In the absence of natural resistance, the use of genetically engineered resistance is an attractive option. The main objective of this study was to develop resistance in banana against banana bunchy top virus through RNAi and the identification of unknown components of BBTV by a new technique called Rolling Circle Amplification (RCA). Rolling circle amplification (RCA) is a novel technique for the amplification of circular DNAs. This technique has been widely used for the amplification of geminiviruses but its use for the characterization of nanoviruses has not been reported. The identification of unknown component is also necessary to find out whether any additional component is associated with infectious unit or not. An analysis of the genetic diversity of BBTV was made by this valuable technique across Tando Jam, Sindh, Pakistan, to characterize components of banana bunchy top virus. The RCA product was digested with several restriction enzymes and was resolved in agarose gel. The resulting RFLP pattern resembled those expected for BBTV. In order to confirm the RFLP analysis, the DNA was probed with cloned components of BBTV. The probes for components DNA-S, DNA-N and DNA-M correctly hybridized to their respective fragment. We further cloned two components of BBTV to verify results. The cloned components were highly homologous to South Pacific group of BBTV as reported from Pakistan. The results of present studies confirmed that RCA technology can be used for characterization of nanoviruses. The technique is of great value to nanovirus research since the components that make up this group are still being discovered. This diversity (low) is also helpful in generating resistance against viruses. So, RNAi construct was made against MRep of BBTV to engineer resistance against BBTV. This construct was transiently checked in banana male flower bud. The buds agro-infiltrated with EHA105 gave better expression as compared to GV3101. Expression of BBTV genes from PVX and under 35S promoter was also observed. Expression of MRep and MP under PVX resulted in necrosis and cell death at the site of inoculation and severe leaf curling and necrosis in newly emerging vii leaves in MP. Clink, NSP and CP produced mild symptoms of leaf curling and mosaic, while CP produced necrotic response in inoculated leaves. When all these genes were expressed under 35S promoter in N. benthamiana 16c line, MP and Clink stabilized GFP specific mRNA and reduced GFP specific siRNA. MRep, NSP and CP did not show accumulation of GFP specific mRNA. These results identified that MP and Clink are supressors of silencing. The ability of MP to induce severe necrosis in inoculated and systemic leaves and RNA silencing suppressors indicates that MP is a major pathogenecity determinant in BBTV genome. Promoter regions of BBTV components may have application for heterologous transgene expression. Promoter regions of BBTV components were cloned in expression vector and checked it in N. benthamiana plants. Out of five components of BBTV, DNA-S, DNA-C and DNA-R did not show any GUS expression in N. benthamiana, while DNA-N showed some level of expression. The deletion of 200bp from 5’ end of DNA-N increased the promoter activity but was still low as compared to CaMV, 35S.