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Home Dialysis / Sample Prep / SPE Liposome Products Liposomat for the Preparation of Large Volume Liposomes


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Liposomat for the Preparation of Large Volume Liposomes
Today liposomes are an important part of biological, pharmaceutical, and medical research. Because liposomes are the most effective
carriers for the introduction of many different types of agents into cells, the applications of liposome-based samples and products are extremely wide.
Liposomat
• The Liposomat is ideal for the preparation of liposomes of volumes from 3 ml to 50 ml or higher.
• The system has two serpentine channels superimposed on each other and separated by a membrane.
• Each channel has a volume of 3 ml and a length of 3 meters. The mixed lipid/detergent micelles run through one of the channels while the buffer flows through the other channel.
• Due to controlled dialysis and the high surface area in the system, liposomes can be formed within 30 minutes.
• The serpentine chambers can also be immersed in a water bath for liposome production at constant temperature.

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Item# Description In Stock Lead Time U.S. List Price Quantity
746400 Liposomat Device for Preparation of Liposomes (3 ml to 50 ml) with Dual Pump, Flow-Through Dialysis Chamber and 100 Membranes (MWCO 5,000 Daltons), qty. of 1 Yes -- View Pricing
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746402 Long Tubing for Use of Liposomat with Thermostat, qty. of 1 Yes -- View Pricing
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Full Description Back to Top

Advantages
• Fast, easy to use
• Unilamellar
• Reproducible
• Uniformly-sized (25 to 800nm)
• Very high encapsulation
• Low lipid loss (1 to 2%)
• Stable liposomes (one year or longer)
Applications
• Drug delivery
• DNA delivery and gene therapy
• Cell-cell interactions
• Cosmetics
• Diagnostics

Today liposomes are an important part of biological, pharmaceutical, and medical research. Because liposomes are the most effective
carriers for the introduction of many different types of agents into cells, the applications of liposome-based samples and products are extremely wide. A few examples are presented below:
• Liposomes are used for studying protein-liposome interactions with compounds such as serum lipoproteins, lectins, toxins and clotting components.
• They are used for the entrapment of anti-tumor agents, anti-microbial drugs, anti-inflammatory and immunomodulatory agents and CNS-active drugs. The therapeutic applications are presently include cancer therapy, arthritis, metal chelation therapy, enzyme replacement therapy, hemophilia (factor VIII), myocardial infarction, and as radiopharmaceutical markers.
• Liposomes are used for studying in vitro and in vivo liposome-cell interactions.
• They are used for reconstitution experiments especially for ion transport systems.
• In molecular biology, liposomes are used for the mediated delivery of macromolecules into eukaryotic cells.
• In immunology, antigens encapsulated in liposomes are used to generate antibodies, to mediate active and passive immunization and for many other applications.
• The use of liposomes in gene-based technology and in broader biotechnology and pharmaceutical applications is increasing day by day.
Harvard Apparatus offers two instruments, the Mini Lipoprep and the Liposomat, for fast, easy and reproducible liposome preparation. No prior experience in liposome preparation is necessary. Using these systems, liposomes can be prepared with virtually any lipid, depending on the specifications of the experiment and the types of biomolecules that need to be encapsulated. Liposome preparation with these instruments is highly reproducible and compared to other liposome preparation methods on the market, these liposomes are very stable. Under sterile conditions, liposomes prepared using the Mini Lipoprep and Liposomat can be stored for one year or longer.
Liposome Specifications
With a few exceptions, liposomes are composed of natural or synthetic phospholipids, mostly lecithins. Hence, they can be metabolized in vivo and are generally non-toxic and non-antigenic.
Agents can be entrapped in liposomes without the formation of chemical bonds and sensitive molecules can be protected within them. Because of their restricted permeability, liposomal preparations offer a controllable, time-dependent release system.
The entrapment of a drug within liposomes changes its pharmaco-kinetics and can result in a better therapeutic index and enhanced cellular uptake. Since different agents need different lipid agents to create an optimal coat, in vivo experiments following liposome preparation are often the optimal means of determining which lipid represents the best compromise between permeability and in vivo stability for any given agent.
Stability of Liposomes
No general rule for maintaining liposome stability exists since it depends on several parameters, such as the type of lipid used, the properties of the drug/agent in the liposomes, their size, lamellarity, and homogeneity, the electrolyte content and pH of the medium used, and also on the specifications of the desired application.
Size Control
The size of liposomes can be adjusted experimentally by varying several parameters: the dialysis rate, type of detergent, type of lipid(s), lipid/detergent molar ratio, lipid concentration, electrolyte content and pH.
Detergents
The detergents used are gentle in their action and are not expected to hydrolyze or peroxidize liposome components. The most frequently used detergents are sodium cholate, n-octyl-b-D-glucopyranoside and n-octyl-tetraoxyethylene (POE4). Other detergents are sodium salts of glycocholic acid, deoxycholic acid, taurocholic acid, chenoxycholic acid, n-hexyl- and n-heptyl-glucopyranoside and lauryldimethylamine oxide.


Journal Articles Back to Top

Displaying 1 to 10 of 11 results for Liposomat for the Preparation of Large Volume Liposomes   Page 1  2 

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Description

100% Login to view VT06 Ventilator use in finding load as an acute determinant of end-diastolic pressure-volume relation.pdf
[200 KB]
h4Ventilator use in finding load as an acute determinant of end-diastolic pressure-volume relation010100051p
37% Login to view Airway Surface Liquid Osmolality Measured using Fluorophore-encapsulated Liposomes.pdf
[258 KB]
Airway Surface Liquid Osmolality Measured during Fluorophore-encapsulated Liposomes
37% Login to view PDMI03 2003microinc.pdf
[251 KB]
Airway Surface Liquid Osmolality Measured during Fluorophore-encapsulated Liposomes
36% Login to view VT34 MRI assessment of LV relaxation by untwisting rate.pdf
[231 KB]
MRI assessment of LV relaxation by untwisting rate
36% Login to view PP57 Quantification of Cerebral Perfusion With Real-Time Contrast-Enhanced Ultrasound.pdf
[210 KB]
Respirator pump use in finding Quantification of Cerebral Perfusion With "Real Time" Contrast-Enhanced Ultrasound
32% Login to view lipomat.pdf
[66 KB]
LipoPrep Instrument used in Engineering Porphyrin Encapsulated Vesicles for Metal Removal from Wastewater
20% Login to view OT12 b2slice2002.pdf
[320 KB]
Independence of extracellular tortuosity and volume fraction during osmotic challenge in rat neocortex
19% Login to view VT06 683 load.pdf
[218 KB]
Animal Ventilator use in finding load as an acute determinant of end-diastolic pressure-volume relation
17% Login to view Independence of extracellular tortuosity.pdf
[331 KB]
Independence of extracellular tortuosity and volume fraction during osmotic challenge in rat neocortex
17% Login to view PP111 pmp.pdf
[395 KB]
Volume controlled pump use in finding Development and Response Timing and Direction Selectivity in Cat Visual Thalamus and Cortex
   

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Manuals Back to Top

Displaying 1 to 1 of 1 result for Liposomat for the Preparation of Large Volume Liposomes  

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100% Login to view Model613 550715.pdf
[270 KB]
Large Animal Volume Controlled Ventilator Manual
   

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