An alternative scheme is proposed to transfer quantum states and prepare a quantum network in cavity QED. It is based on the interaction of a two-mode cavity field with a three-level V-type atom. In the scheme, the at...An alternative scheme is proposed to transfer quantum states and prepare a quantum network in cavity QED. It is based on the interaction of a two-mode cavity field with a three-level V-type atom. In the scheme, the atom-cavity field interaction is resonant, thus the time required to complete the quantum state transfer process is greatly shortened, which is very important in view of decoherence. Moreover, the present scheme does not require one mode of the cavities to be initially prepared in one-photon state, thus it is more experimentally feasible than the previous ones.展开更多
In the present research,enzyme encapsulated hydrogels(single gels and double network gels)and enzyme immobilized magnetic beads,which allow high-throughput screening,were fabricated and evaluated in terms of the pre...In the present research,enzyme encapsulated hydrogels(single gels and double network gels)and enzyme immobilized magnetic beads,which allow high-throughput screening,were fabricated and evaluated in terms of the preservation,precision, and repeatability of enzyme activity.The fabricated gels and magnetic beads were analyzed in a 96-well microassay plate.Trypsin was successfully encapsulated in both types of gels and immobilized to the magnetic beads.However,pepsin,either encapsulated in the gels or immobilized to the magnetic beads,could not react with its substrates.The adaptability to various enzymes (e.g.,trypsin,β-glucuronidase,and CYP1A1)in the single gels and magnetic beads was superior to that in double network gels.However,the soak out of the enzymes was observed in the single gels.The double network gels could encapsulate trypsin,whereas the fabrication of the other enzymes(e.g.β-glucuronidase,CYP1A1,and pepsin)failed because of the inactivation of the enzymes by acryl amide and ammonium peroxodisulfate,which are the components of the gel formulation. The enzyme reaction in the magnetic beads exhibited the highest efficiency among the three fabrication methods.Furthermore, the stability of the enzymes immobilized to the magnetic beads was better than that fabricated by the other methods,and the activities of trypsin andβ-glucuronidase did not decline for up to one week.In addition,in the magnetic beads,the activities of trypsin andβ-glucuronidase can be well repeated.Hence,although the adaptability of the double network gels to various enzymes is currently limited,the efficiency of the enzyme encapsulation can be improved by optimizing the formulation of acryl amide gels.展开更多
基金The project supported by National Natural Science Foundation of China under Grant Nos. 10225421 and 10674025
文摘An alternative scheme is proposed to transfer quantum states and prepare a quantum network in cavity QED. It is based on the interaction of a two-mode cavity field with a three-level V-type atom. In the scheme, the atom-cavity field interaction is resonant, thus the time required to complete the quantum state transfer process is greatly shortened, which is very important in view of decoherence. Moreover, the present scheme does not require one mode of the cavities to be initially prepared in one-photon state, thus it is more experimentally feasible than the previous ones.
基金The Global COE Program from the Ministry of Education,Science,Sports,and Culture of Japan.
文摘In the present research,enzyme encapsulated hydrogels(single gels and double network gels)and enzyme immobilized magnetic beads,which allow high-throughput screening,were fabricated and evaluated in terms of the preservation,precision, and repeatability of enzyme activity.The fabricated gels and magnetic beads were analyzed in a 96-well microassay plate.Trypsin was successfully encapsulated in both types of gels and immobilized to the magnetic beads.However,pepsin,either encapsulated in the gels or immobilized to the magnetic beads,could not react with its substrates.The adaptability to various enzymes (e.g.,trypsin,β-glucuronidase,and CYP1A1)in the single gels and magnetic beads was superior to that in double network gels.However,the soak out of the enzymes was observed in the single gels.The double network gels could encapsulate trypsin,whereas the fabrication of the other enzymes(e.g.β-glucuronidase,CYP1A1,and pepsin)failed because of the inactivation of the enzymes by acryl amide and ammonium peroxodisulfate,which are the components of the gel formulation. The enzyme reaction in the magnetic beads exhibited the highest efficiency among the three fabrication methods.Furthermore, the stability of the enzymes immobilized to the magnetic beads was better than that fabricated by the other methods,and the activities of trypsin andβ-glucuronidase did not decline for up to one week.In addition,in the magnetic beads,the activities of trypsin andβ-glucuronidase can be well repeated.Hence,although the adaptability of the double network gels to various enzymes is currently limited,the efficiency of the enzyme encapsulation can be improved by optimizing the formulation of acryl amide gels.
