Expression and purifcation of thermostable alkaline phosphatase produced by genetic engineering;

The concentration of POS was tested by alkaline phosphatase,this way was proved to be dependable.

The susceptibility of Tessaratoma papillosa to trichlorphon was tested with topical application method,and the effect of trichlorphon on carboxylesterase,acid phosphatase and alkaline phosphatase was studied.

Objective To contrast difference between the effect of various concentrations DDVP and nanoemulsion to the acetylcholine esterase(AchE),glutathione-s-transferase(GST) and base phosphastase(BpE) activity of Blattella germanica.

Objective: To study the relationship between the activities of carboxylesterase、 acid phosphastase、 base phosphastase and pesticide resistance in the German cockroach.

In order to determine the functional domain of thermostable alkaline phosphatase(TAPND27),three truncators of pTAPN8,pTAPN16 and pTAPN25 with deletions of 8,16 and 25 amino acids at N\|terminal and two truncators of pTAPC10 and pTAPC30 with deletions of 10 and 30 amino acids at C\|terminal were obtained through PCR\|mediated site\|directed mutagenesis.

To reveal the mechanism of protein thermostability, we used in vivo random mutagenesis to generate variants of PTAP503F which contained thermostable alkaline phosphatase (FD-TAP).

The coding sequence of the gene for recombinant thermostable alkaline phosphatase (FD-TAP) was amplified from the pTAP118B by polymerase chain reaction (PCR) using two mutagenic primers incorporating Nde I and Burn H I sites at the 5 termini,respectively.

The coding sequence of the gene for human placental alkaline phosphatase(PLAP)was amplified from the pSEAP2-control plasmid by polymerase chain reaction(PCR).