Literature DB >> 1548405

Post-formation fluorescent labelling of liposomal membranes. In vivo detection, localisation and kinetics.

E Claassen1.   

Abstract

A fast and simple method for the in vivo/in situ detection of liposomes is described. Utilizing lipophilic carbocyanine dyes, DiI and DiO, yellow (or red) and green fluorescent liposomes can be visualised with routinely available filters. The main advantages of the method are (i) the vesicles can be labelled after they are formed and (ii) the label does not interfere with proteins on the surface of the liposomes. Labelled liposomes were found in macrophages of spleen and liver (of mice) within 30 min of intravenous administration. In the spleen, labelled liposomes localised preferentially in the marginal zone macrophages, as confirmed by double staining with FITC-Ficoll. These data correlate well with the fact that empty or haptenated liposomes are thymus-independent antigens, and that other thymus-independent antigens are also specifically taken up by marginal zone macrophages. The immunological role of these macrophages in the processing and presentation of antigen-bearing liposomes can now be studied in more detail. Administration of high doses (1-3 mg lipid) of labelled liposomes showed that uptake occurred preferentially, but not exclusively, by marginal zone macrophages. After the marginal zone macrophages had been 'saturated', the red pulp macrophages took up the liposomes. DiI and DiO have also been successfully used for labelling lymphocytes and bacteria for in vivo homing studies. The fact that liposomes can be labelled after they have been formed is an advantage for retrospective (i.e. liposomes already in use/storage) studies in e.g. targeting of drugs by liposomes.

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Year:  1992        PMID: 1548405     DOI: 10.1016/s0022-1759(12)80013-5

Source DB:  PubMed          Journal:  J Immunol Methods        ISSN: 0022-1759            Impact factor:   2.303


  7 in total

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Authors:  Tatjana Nikolic; Dowty Movita; Margaretha E H Lambers; Claudia Ribeiro de Almeida; Paula Biesta; Kim Kreefft; Marjolein J W de Bruijn; Ingrid Bergen; Niels Galjart; Andre Boonstra; Rudi Hendriks
Journal:  Cell Mol Immunol       Date:  2013-09-09       Impact factor: 11.530

2.  Tolerogenic nanoparticles suppress central nervous system inflammation.

Authors:  Jessica E Kenison; Aditi Jhaveri; Zhaorong Li; Nikita Khadse; Emily Tjon; Sara Tezza; Dominika Nowakowska; Agustin Plasencia; Vincent P Stanton; David H Sherr; Francisco J Quintana
Journal:  Proc Natl Acad Sci U S A       Date:  2020-11-25       Impact factor: 11.205

3.  Macrophage depletion in the rat after intraperitoneal administration of liposome-encapsulated clodronate: depletion kinetics and accelerated repopulation of peritoneal and omental macrophages by administration of Freund's adjuvant.

Authors:  J Biewenga; M B van der Ende; L F Krist; A Borst; M Ghufron; N van Rooijen
Journal:  Cell Tissue Res       Date:  1995-04       Impact factor: 5.249

4.  A robust and quantitative method for tracking liposome contents after intravenous administration.

Authors:  Aditya G Kohli; Heidi M Kieler-Ferguson; Darren Chan; Francis C Szoka
Journal:  J Control Release       Date:  2013-12-22       Impact factor: 9.776

5.  Killing of Entamoeba invadens using liposome-encapsulated drugs.

Authors:  N van Rooijen; J Bakker; A Sanders; J Mellink
Journal:  Parasitol Res       Date:  1995       Impact factor: 2.289

6.  Reversible depletion of synovial lining cells after intra-articular treatment with liposome-encapsulated dichloromethylene diphosphonate.

Authors:  P L van Lent; L van den Bersselaar; A E van den Hoek; M van de Ende; C D Dijkstra; N van Rooijen; L B van de Putte; W B van den Berg
Journal:  Rheumatol Int       Date:  1993       Impact factor: 2.631

7.  Following the Fate of Dye-Containing Liposomes In Vitro.

Authors:  Jennifer Cauzzo; Mona Nystad; Ann Mari Holsæter; Purusotam Basnet; Nataša Škalko-Basnet
Journal:  Int J Mol Sci       Date:  2020-07-09       Impact factor: 5.923

  7 in total

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