The human lactoferrin (hLF) is a component of the immune system. In this study, immunofluorescence assays are used to demonstrate both the hepatocellular uptake of hLF and a qualitative reduction in the hepatitis C virus replication upon treatment with hLF.
Imunofluorescência é uma técnica de laboratório vulgarmente usados para estudar vários aspectos da biologia. É tipicamente usado para visualizar a distribuição e / ou a localização de uma molécula alvo em células e tecidos. Imunofluorescência baseia-se na especificidade de anticorpos fluorescentes marcado contra os seus antigénios correspondentes no interior de uma célula. Ambas abordagens directas e indirectas de imunofluorescência pode ser usado que se baseiam no uso de anticorpos ligados a um fluorocromo. A imunofluorescência direta é menos freqüentemente usado porque fornece sinal inferior, envolve custos mais elevados e menos flexibilidade. Em contraste, imunofluorescência indireta é mais comumente utilizado devido à sua alta sensibilidade e fornece um sinal amplificado desde mais de um anticorpo secundário pode anexar a cada anticorpo primário. Neste texto, tanto microscopia de epifluorescência e microscopia confocal foi utilizada para monitorizar a internalização da lactoferrina humana, um componente importante da resposta imunesistema, em células hepáticas. Além disso, nós monitorizado o potencial inibitório da hLF na replicação intracelular do vírus da hepatite C por meio de imunofluorescência. Ambas as vantagens e desvantagens associadas a estes métodos são discutidos.
Immunofluorescence is a technique that uses a fluorescence microscope to visualize the distribution and/or localization of a target molecule in a biological sample. Immunofluorescence relies on the specificity of fluorescent-labelled antibodies against their corresponding antigens within a cell1. It is typically used on tissue sections and cultured cell lines in order to analyze the distribution/localization of various biological molecules such as proteins, nucleic acids and glycans. It should be noted that immunofluorescence is often used in combination with other non-antibody methods of fluorescent staining such as the 4′,6-diamidino-2-phenylindole (DAPI) stains which are typically used to label DNA2. Moreover, this technique involves fixation of the cells which allows the analysis of cells at a specific time.
Different types of microscopes can be used to analyze immunofluorescence samples. The simplest is the epifluorescence microscope (Figure 1) for which excitation of the fluorochrome and detection of the fluorescence are done through the same light path3. Because most of the excitation light is transmitted through the sample, only reflected excitatory light can reach the objective together with the emitted light. This approach unfortunately leadsto a frequent high signal to noise ratio.In contrast, confocal microscopy (Figure 2) offers a distinct advantage for increasing optical resolution and contrast by means of adding a spatial pinhole placed at the confocal plane of the lens to eliminate out-of-focus light4. This approach allows the reconstruction of three-dimensional structures from the obtained images. However, since an important fraction of the light from the sample is blocked at the pinhole, long exposures are often required.
There are two classes of immunofluorescence techniques, primary (or direct) and secondary (or indirect). Direct immunofluorescence involves a primary antibody linked with a fluorochrome (Figure 3). This method is less frequently used because it provides lower signal, involves higher cost and less flexibility1. Moreover, such antibodies are generally harder to find commercially. On the other hand, the direct attachment of the fluorochrome to the antibody significantly reduces the number of steps in the procedure, saving time and frequently reducing non-specific background signal. This also limits the possibility of antibody cross-reactivty.
Indirect immunofluorescence involves a primary unlabelled antibody which is specific for the epitope of interest1. A secondary antibody which carries the fluorochrome then recognizes the primary antibody and binds to it (Figure 3). Although indirect immunofluorescence is more complex and time consuming than direct immunofluorescence, it is frequently used because of its high sensitivity and it also provides an amplified signal since more than one secondary antibody can attach to each primary antibody. In addition, a vast array of commercial secondary antibodies is available at affordable prices.
Hepatitis C virus (HCV) is a major public-health problem with 130-170 million individuals chronically infected worldwide. In order to halt the epidemic, therapy against HCV will need to be both effective and widely available. Studies focusing on safe and affordable natural product active against HCV have revealed the antiviral activity of the human Lactoferrin (hLF) protein which binds and neutralizes the circulating virion5. In the current study, investigation of hLF activity on the HCV subgenomic replicon system, which is independent from viral entry and shedding, revealed a distinct antireplicative activity of hLF against HCV. This manuscript presents a study in which immunofluorescence assays were performed to monitor the internalization of hLF, an important component of the immune system6, into hepatic cells. Moreover, we monitored the inhibitory potential of hLF on the intracellular replication of the Hepatitis C virus (HCV).
A epidemia de HCV permanece uma ameaça global, com 80% dos pacientes recém-infectadas desenvolvem uma infecção crônica, colocando-os em risco de cirrose, insuficiência hepática ou carcinoma hepatocelular. Por acção directa agentes antivirais combatem a replicação do HCV e maturação representam agentes anti-HCV de primeira linha, como recentemente demonstrado pela aprovação regulamentar de dois NS3 N-terminal inibidores da protease (boceprevir e telaprevir). A actividade anti-VHC hLF é actualmente acredit…
The authors have nothing to disclose.
This work was funded by both the Canadian Institutes of Health Research and Natural Sciences and the Engineering Research Council of Canada. M. Bisaillon is a Chercheur Boursier Senior from the Fonds de Recherche en Santé du Québec and also a member of the Centre de Recherche Clinique du Centre Hospitalier Universitaire de Sherbrooke. We thank Dr. Ralf Bartenschlager for the generous gift of the HCV replicon system. We also thank Dr. Charles Rice and Dr. Daniel Lamarre for kindly providing the hepatic cell line. We also want to thank Guillaume Tremblay for technical assistance.
DMEM | Wisent | 319-005-CL | |
PAF | BioShop | PAR070.1 | Flammable solid, skin irritant, lungs and eyes. |
PBS | Wisent | 311-425-CL | Without Ca2+ & Mg2+ |
NGS | Wisent | 053-150 | |
AlexaFluor 488-labeled anti-mouse | Invitrogen | A11017 | |
AlexaFluor 568-labeled anti-rabbit | Invitrogeb | A21069 | |
Wheat germ agglutinin Alexa Fluor 488 conjugate (WGA) | Invitrogen | W11261 | Potentially mutagenic |
Anti-NS5A rabbit | Abcam | ab2594 | |
Anti-hLF mouse | Abcam | ab10110 | |
SlowFade | Invitrogen | S36937 | |
Hoechst stain | Life Techn. | H1399 | Potentially mutagenic and carcinogenic |
hLF | Sigma | L0520 | |
Nikon Eclipse visible/epifluorescence Microscope | Nikon | TE2000-E | |
epifluorescence/confocal microscope | Olympus | FV1000 |