269 MOLECULAR REQUIREMENTS FOR VLA-4-MEDIATED B-LYMPHOCYTE ADHERENCE UNDER FLOW CONDITIONS. Issue 1 (1st January 2007)
- Record Type:
- Journal Article
- Title:
- 269 MOLECULAR REQUIREMENTS FOR VLA-4-MEDIATED B-LYMPHOCYTE ADHERENCE UNDER FLOW CONDITIONS. Issue 1 (1st January 2007)
- Main Title:
- 269 MOLECULAR REQUIREMENTS FOR VLA-4-MEDIATED B-LYMPHOCYTE ADHERENCE UNDER FLOW CONDITIONS.
- Authors:
- Mills, D. A.
Brown, D. C.
Ramirez, S.
Chigaev, A.
Sklar, L. A.
Laurence, M.
Larson, R. S. - Abstract:
- Abstract : VLA-4 is critical for normal lymphocyte recirculation. Expressed on B lymphocytes, VLA-4 binds VCAM-1 on endothelium as a first step in lymphocyte extravasation. In this study, we examine the behavior of B lymphocytes on purified VCAM-1 as a first step toward quantifying the molecular parameters and requirements for lymphocyte rolling and arrest mediated by VLA-4. In our first set of observations, we wished to define chemokines that stimulated VLA-4 on human B lymphocytes isolated from blood and determine the site densities over which VLA-4-mediated attachment could occur. We tested a panel of chemokines and show that four chemokines may stimulate VLA-4 activation on human peripheral blood B lymphocytes. We next show that B lymphocytes isolated from peripheral blood will roll and attach to VCAM-1 in the absence of cellular stimulation; B-lymphocyte accumulation does not occur below 50 sites/μm 2 of VCAM-1 and shows increasing accumulation up to 200 sites/mm 2 . Interestingly, VLA-4 is activated to its high-affinity state using Mn 2+ or SDF-1α stimulation, and increased accumulation is seen over the range of 50 to 200 sites/μm 2 compared with no cellular stimuli, yet the site density over which attachment occurs remains unchanged. We then examined the effect of culturing B lymphocytes after isolation from blood on VLA-4-mediated binding. Using a VCAM-1 site density that would promote maximal binding (≈1, 200 sites/μm 2 ), we show that the proportion ofAbstract : VLA-4 is critical for normal lymphocyte recirculation. Expressed on B lymphocytes, VLA-4 binds VCAM-1 on endothelium as a first step in lymphocyte extravasation. In this study, we examine the behavior of B lymphocytes on purified VCAM-1 as a first step toward quantifying the molecular parameters and requirements for lymphocyte rolling and arrest mediated by VLA-4. In our first set of observations, we wished to define chemokines that stimulated VLA-4 on human B lymphocytes isolated from blood and determine the site densities over which VLA-4-mediated attachment could occur. We tested a panel of chemokines and show that four chemokines may stimulate VLA-4 activation on human peripheral blood B lymphocytes. We next show that B lymphocytes isolated from peripheral blood will roll and attach to VCAM-1 in the absence of cellular stimulation; B-lymphocyte accumulation does not occur below 50 sites/μm 2 of VCAM-1 and shows increasing accumulation up to 200 sites/mm 2 . Interestingly, VLA-4 is activated to its high-affinity state using Mn 2+ or SDF-1α stimulation, and increased accumulation is seen over the range of 50 to 200 sites/μm 2 compared with no cellular stimuli, yet the site density over which attachment occurs remains unchanged. We then examined the effect of culturing B lymphocytes after isolation from blood on VLA-4-mediated binding. Using a VCAM-1 site density that would promote maximal binding (≈1, 200 sites/μm 2 ), we show that the proportion of VLA-4-expressing B lymphocytes that roll on VCAM-1 progressively increases from 1 to 4 days of culture (90% firm arrest/10% rolling on day 1 versus 45% firm arrest/55% rolling on day 4). Flow cytometry-based site density experiments indicate that the VLA-4 site density on B cells remains constant over the 4 days. To determine whether the change in VLA-4-mediated rolling and arrest on VCAM-1 was due to changes in the native receptor affinity or intracellular signaling, we performed a series of studies of pharmacologic studies. Exposure of day 1 or day 4 B lymphocytes to Mn 2+ and DTT, activators of VLA-4, promoted firm attachment of greater than 90% of the cells, indicating that VLA-4 could obtain a high-affinity state regardless of culture duration. Inhibition of protein kinase C, farnesyl transferase, and G protein-coupled receptor signaling increases the proportion of rolling cells with fewer overall attachments. This phenomenon is observed on day 1 and is more pronounced on day 4, suggesting that inside-out signaling remains intact despite culturing. In all, we quantify for the first time the effect of site density and postisolation culture on the behavior of VLA-4-mediated adherence of B lymphocytes. Our observations also suggest that signaling both from and to the VLA-4 receptor occurs and changes during postisolation culture. These observations are important in resolving previous studies examining VLA-4-mediated lymphocyte rolling and arrest. … (more)
- Is Part Of:
- Journal of investigative medicine. Volume 55:Issue 1(2007)
- Journal:
- Journal of investigative medicine
- Issue:
- Volume 55:Issue 1(2007)
- Issue Display:
- Volume 55, Issue 1 (2007)
- Year:
- 2007
- Volume:
- 55
- Issue:
- 1
- Issue Sort Value:
- 2007-0055-0001-0000
- Page Start:
- S120
- Page End:
- S120
- Publication Date:
- 2007-01-01
- Subjects:
- Clinical medicine -- Periodicals
Medicine -- Research -- Periodicals
Medicine
Research -- United States
Clinical medicine
Medicine -- Research
Periodicals
616.075 - Journal URLs:
- http://journals.lww.com/jinvestigativemed/pages/default.aspx ↗
http://jim.bmj.com/ ↗
https://journals.sagepub.com/home/IMJ ↗
http://journals.lww.com ↗ - Languages:
- English
- ISSNs:
- 1081-5589
- Deposit Type:
- Legaldeposit
- View Content:
- Available online (eLD content is only available in our Reading Rooms) ↗
- Physical Locations:
- British Library DSC - 5008.010000
British Library DSC - BLDSS-3PM
British Library STI - ELD Digital store - Ingest File:
- 17619.xml