Nanthanit Jaruseranee

Nanthanit Jaruseranee
Mae Fah Luang University | MFU · School of Science

About

7
Publications
5,195
Reads
How we measure 'reads'
A 'read' is counted each time someone views a publication summary (such as the title, abstract, and list of authors), clicks on a figure, or views or downloads the full-text. Learn more
288
Citations
Introduction
Skills and Expertise
Phage Display
Phage Display Technology
Recombinant Antibodies
Antibody Engineering
Monoclonal Antibodies
Recombinant Protein Expression
Monoclonal Antibody Production
Antibody Discovery
Protein Expression
Epitope Mapping

Publications

Publications (7)
Synthetic construct DNA helicase RecQ (recQ1) gene, complete cds
Data
  • Jul 2014
##Assembly-Data-START## Sequencing Technology :: Sanger dideoxy sequencing ##Assembly-Data-END##
View
Formation of chitin-based nanomaterials using a chitin-binding peptide selected by phage-display
Article
  • Mar 2012
Targeting polymers with peptides is an efficient strategy to functionalize biomaterials. Phage display technology is one of the most powerful techniques for selecting specific peptides for a wide variety of targets. A method to select a chitin-binding peptide from a 12-mer random peptide library was successfully performed against chitin immobilized...
View
Table 1 Overview of selection of antibodies against aflatoxin B1-BSA 
Table 2 Percentage cross-reactivity values of the TomI-F6 and YM1-C3...
Fig. 2 Amino acids sequence analysis The amino acid sequence of the...
One-Step Detection of Aflatoxin-B1 Using scFv-Alkaline Phosphatase-Fusion Selected from Human Phage Display Antibody Library
Article
Full-text available
  • Apr 2011
A unique human phage display library was used to successfully generate a scFv to the highly carcinogenic toxin aflatoxin B1. Such an antibody has major potential applications in therapy and diagnostics. To further exploit its analytical capacity, the scFv was genetically fused to alkaline phosphatase, thereby generating a novel and highly sensitive...
View
Figure 1. Map of the two expression vectors. The structure of plasmids...
Figure 2. Zymogram analysis of the recombinant B. subtilis β-mannanase...
Efficient E. coli expression systems for the production of recombinant ??-mannanases and other bacterial extracellular enzymes
Article
Full-text available
  • Jan 2011
Two Escherichia coli expression systems based on T7 RNA polymerase promoter (pET system) and tac promoter (pFLAG system) have been used for the production and secretion of recombinant β-mannanases from Bacillus sp. Both E. coli OmpA signal peptide and native Bacillus signal peptide could be used efficiently for the secretion of recombinant enzymes...
View
Table 2 : Results of affinity selections with different targets
Map of phagemid vector, pMod1, for the construction of scFv...
Schematic outline of the strategy used for the construction of compact...
DNA fingerprinting of random clones from unselected library. Fifteen...
+1 Binding specificity of selected phage. Panel A shows the specific...
A compact phage display human SCFV library for selection of antibodies to a wide variety of antigens
Article
Full-text available
  • Feb 2009
Phage display technology is a powerful new tool for making antibodies outside the immune system, thus avoiding the use of experimental animals. In the early days, it was postulated that this technique would eventually replace hybridoma technology and animal immunisations. However, since this technology emerged more than 20 years ago, there have onl...
View
Additional File 1
Data
Full-text available
  • Jan 2009
Amino acids sequences of ten random clones from unselected library. Amino acid sequence and germ line family of ten random clones from unselected library.
View
Secretion of recombinant Bacillus hydrolytic enzymes using Escherichia coli expression systems
Article
  • Feb 2008
Bacillus spp. are Gram-positive bacteria that secrete a large number of extracellular proteins of industrial relevance. In this report, three Bacillus extracellular hydrolytic enzymes, i.e., alpha-amylase, mannanase and chitinase, were cloned and over-expressed in Gram-negative Escherichia coli. We found that both the native signal peptides and tha...
View

Network

Cited
View All
Cited By
View All