Comparison of two automated DNA amplification systems with culture fordetection of Chlamydia trachomatis and Neisseria gonorrhoeaeinfections in symptomatic men

邱莊儀, Yau, Chong-yee, Miranda.

January 2000

published_or_final_version / Medical Sciences / Master / Master of Medical Sciences

Gene amplification.

Polymerase chain reaction.

Chlamydia trachomatis - Diagnosis.

Gonorrhea - Diagnosis.

Evaluation of a multiplex polymerase chain reaction assay for detection of silent fluoroquinolone-resistant determining mutations instreptococcus pneumoniae

Cheung, Yin-mei., 張燕湄.

January 2003

published_or_final_version / Medical Sciences / Master / Master of Medical Sciences

Polymerase chain reaction - Evaluation.

Drug resistance.

Multiplex RT-PCR for typing and subtyping influenza and respiratory syncytial viruses

劉永棠, Lau, Wing-tong, Ricky.

January 2002

published_or_final_version / Medical Sciences / Master / Master of Medical Sciences

Respiratory syncytial virus.

Influenza viruses.

Viral genetics.

Polymerase chain reaction.

Reverse transcriptase.

Quantitative analysis of hTERT mRNA expression in gestational trophoblastic disease by real-time PCR

張綺雲, Cheung, Yee-wan.

January 2002

published_or_final_version / Medical Sciences / Master / Master of Medical Sciences

Trophoblastic tumors - Genetic aspects.

Telomerase.

Messenger RNA.

Polymerase chain reaction.

Gene expression.

The development and assessment of assays for quantitation of hepatitisB virus DNA (HBV DNA) and the clinical significance of low HBV DNAlevel in patients with chronic hepatitis B

Sum, Siu-man, Simon., 岑紹文.

January 2004

published_or_final_version / abstract / toc / Medicine / Master / Master of Philosophy

Hepatitis B virus.

Hepatitis B - Genetic aspects.

Study on the use of potential prognostic parameters in breast cancer patients

胡夕春, Hu, Xichun.

January 2001

published_or_final_version / abstract / toc / Surgery / Doctoral / Doctor of Philosophy

Genetic transcription.

Polymerase chain reaction.

Tumor markers - Diagnostic use.

Breast - Cancer - Genetic aspects.

Metastasis.

Population genetics study on the variable number of Tandem repeats (VNTR) loci of a Han Chinese population in Hong Kong and itsapplication in human identity

Ng, Sau-wah., 吳秀華.

January 2000

published_or_final_version / Pathology / Master / Master of Philosophy

Polymerase chain reaction.

Biochemical markers.

Development of an expression system for a dehydrogenase

Veibäck, Axel

January 2010

In recent years, biocatalytical steps in chemical synthesis are becoming increasingly important for economical and environmental-friendly production. In order to evaluate the use of enzymes in a process at Cambrex Karlskoga AB, an expression system was developed for a dehydrogenase. A synthetic gene was cloned into Escherichia coli DH5a cells, using the pTZ19R expression vector, as previously described in the literature. Protein expression was carried out at 25°C, 30°C and 37°C and results were measured using SDS-PAGE and activity assays. To improve expression, the gene was modified in three ways using PCR, yielding eight clones: It was inserted into the pSE420 expression vector, shortened to avoid inclusion body formation and a missing nucleotide was inserted into the sequence. A protocol for inclusion body screening was also developed. Finally, an assay for determining the kinetic constants of dehydrogenase was designed. It is concluded that further experiments must be done to obtain expression of the dehydrogenase and recommendations for additional work are given. / Biokatalytiska processteg har de senaste åren blivit ett allt viktigare inslag i kemisk syntes för att åstadkomma ekonomisk och miljövänlig produktion. För att utvärdera användandet av enzymer i en process hos Cambrex Karlskoga AB utvecklades ett expressionssystem för ett dehydrogenas. En syntetisk gen klonades in i Escherichia coli DH5a och uttrycktes med hjälp av expressionsvektorn pTZ19R, som tidigare finns beskrivet i litteraturen. Proteinuttrycket utfördes vid 25°C, 30°C och 37°C och resultatet mättes med hjälp av SDS-PAGE och aktivitetsmätningar. Genen för dehydrogenaset modifierades på tre sätt, vilket gav upphov till åtta varianter. Genen fördes över till expressionsvektorn pSE420, kortades för att undvika bildning av inklusionskroppar och en nukleotid som fattades från gensekvensen återinfördes. Ett protokoll utarbetades även för undersökning av inklusionskroppar. Till sist sammanställdes en metod för att undersöka de kinetiska konstanterna hos dehydrogenaset. Slutsatsen av arbetet är att fortsatta studier måste utföras för att erhålla uttryck av dehydrogenaset och rekommendationer ges för framtida undersökningar.

biocatalysis

protein expression

gene expression

inclusion bodies

SDS-PAGE

polymerase chain reaction

pTZ19R

pSE420

Biochemistry

Biokemi

Scalable, modular, integrated genetic analysis systems

Bidulock, Allison Christel Elizabeth

Unknown Date

No description available.

genetic analysis system

modular

scalable

capillary electrophoresis

polymerase chain reaction

microfluidics

integrated

VLSI Design and System Integration for a USB Genetic Amplification Platform

Ho, Sunny

Unknown Date

No description available.

VLSI

USB

polymerase chain reaction

genetic amplification

microfluidic system

biomedical

lab-on-a-chip