Gene transfection by quantitatively reconstituted Sendai envelope proteins into liposomes

Kim, Hong Sung; Park, Yong Serk

doi:10.1038/sj.cgt.7700421

Cited by 11 publications

(5 citation statements)

References 23 publications

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“…Recently we also reported that negatively-charged PS that contained Sendai virosomes efficiently transfer genes into cultured cells (Kim and Park, 2002). However, among the electron negatively-charged virosomes, the ASVE-and PSvirosomes were relatively efficient in gene transfer while the PA-virosomes were not (Fig.…”

Section: In Vitro Gene Transfer Mediated By F/hn-virosomes Of Varied mentioning

confidence: 98%

“…The fusogenic proteins that were reconstituted into the virosomes were another major factor that governed transfection efficiency. In this study, the F/HN-proteins were reconstituted at a 1 : 100 weight ratio of protein to lipid, the ratio at which in vitro gene transfection has been found to be the most efficient (Kim and Park, 2002).…”

Section: In Vitro Gene Transfer Mediated By F/hn-virosomes Of Varied mentioning

confidence: 99%

“…Tel: 82-33-760-2448;Fax: 82-33-763-5224 E-mail: yspark@dragon.yonsei.ac.kr Recently, we reported that the Sendai virosomes were an efficient vector for transferring the gene into 293 cells (Kim and Park, 2002). Virosomal constituents, such as the lipid components and their molar ratios, and the concentrations of viral envelope proteins can dramatically affect the efficiency of the gene transfer that is mediated by Sendai virosomes (Kaneda et al, 1999;Ponimaskin et al, 2000).…”

Section: Introductionmentioning

confidence: 99%

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Effect of Lipid Compositions on Gene Transfer into 293 Cells Using Sendai F/HN-virosomes

Kim

Park²

2002

BMB Reports

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Section: In Vitro Gene Transfer Mediated By F/hn-virosomes Of Varied mentioning

confidence: 98%

Section: In Vitro Gene Transfer Mediated By F/hn-virosomes Of Varied mentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Effect of Lipid Compositions on Gene Transfer into 293 Cells Using Sendai F/HN-virosomes

Kim

Park²

2002

BMB Reports

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“…Moreover lipid vesicles also do not release the incorporated molecule instantaneously so they can act as local depot for sustained release of drug or immunogen. Some commonly employed vesicular carriers that facilitate permeation includes liposomes [5,63], niosomes [5,63,64], transfersomes [63,65], virosomes [66] Reconstituted Sandai Virus Envelop (RSVE) [69][70] etc. The driven forces, which are involved in selective transfer of lipid vesicles through intact skin, are osmotic gradient and hydration force generally.…”

Section: Transfersomes Niosomes and Liposomesmentioning

confidence: 99%

A Needle-Free Approach for Topical Immunization: Antigen Delivery via Vesicular Carrier System(s)

Mahor

Gupta²,

Rawat³

et al. 2007

CMC

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Topical immunization (TI) is novel and needle free strategy involving vaccine delivery through topical application of antigen and adjuvant(s) directly or via a suitable carrier system on intact skin. Anatomy and physiology of skin attracts scientists in developing topical carrier system(s) for enhanced delivery of bioactive(s). Numerous techniques i.e. physical, chemical and vesicular carrier systems have been exploited for topical immunization. The present review discuss various vesicular systems i.e. liposomes, niosomes, transfersomes, vesosomes etc. for the efficient topical delivery of various immunogens along with comparative points of their merit(s) in TI. The mechanism of permeation of bioactive(s) through skin route via these carriers to the immune system for development of both cellular and humeral immunity has also been discussed. Moreover, the effect of composition and type of carrier system on type of immunity induced has also been focused to develop new effective carrier system(s) for topical immunization.

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“…15 We have developed a novel Sendai F/HN virosome system for in vivo gene transfection. The Sendai virosome formulations were optimized for in vitro and in vivo transfection, especially systemic gene delivery.…”

Section: Introductionmentioning

confidence: 99%

An efficient liposomal gene delivery vehicle using Sendai F/HN proteins and protamine

Kim

Lee

et al. 2008

Cancer Gene Ther

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By means of a simple mixing procedure, we have constructed cationic Sendai virosomes consisting of fusogenic viral F/HN proteins and cationic lipids. Sendai virus F/HN proteins were purified by Triton X-100 treatment and sequential centrifugation, and then quantitatively added to cationic liposomes. The presence of HN proteins is essential for hemolytic activity of Sendai virus as well as efficient gene transfection. The amount of detergent added for purification of F/HN proteins was also crucial for hemolytic activity. The relevance of F/HN proteins in the gene-transfer capability of the cationic Sendai F/HN virosomes (CSVs) was verified by heat inactivation of the F/HN proteins, and cell-binding competition. DNA condensation by protamine sulfate was able to further enhance the transfection efficiency and serum resistance of CSV. The enhanced transfection efficiency of protamine-condensed DNA-encapsulating cationic Sendai F/HN virosomes (PCSVs) may result from specific and efficient cell binding mediated by F/HN proteins and efficient DNA encapsulation by protamine. The DNA condensation by protamine was crucial for systemic in vivo gene transfer by CSVs. The PCSVs exhibited a higher gene expression in various organs, especially the liver, compared to DOTAP/Chol lipoplexes. These results demonstrate the potential for the use of PCSV as gene delivery vehicles for systemic gene transfer.

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Gene transfection by quantitatively reconstituted Sendai envelope proteins into liposomes

Cited by 11 publications

References 23 publications

Effect of Lipid Compositions on Gene Transfer into 293 Cells Using Sendai F/HN-virosomes

Effect of Lipid Compositions on Gene Transfer into 293 Cells Using Sendai F/HN-virosomes

A Needle-Free Approach for Topical Immunization: Antigen Delivery via Vesicular Carrier System(s)

An efficient liposomal gene delivery vehicle using Sendai F/HN proteins and protamine

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