(Received for publication, November 18, 1996, and in revised form, December 23, 1996)
From the Division of Pulmonary and Critical Care Medicine, Department of Internal Medicine, University of Michigan, Ann Arbor, Michigan 48109-0652
5-Lipoxygenase catalyzes the synthesis of leukotrienes from arachidonic acid. The subcellular distribution of 5-lipoxygenase is known to be cell type-dependent and is cytosolic in blood neutrophils. In this study, we asked whether neutrophil recruitment into sites of inflammation can alter the subcellular compartmentation of 5-lipoxygenase. In peripheral blood neutrophils from rats, 5-lipoxygenase was exclusively cytosolic, as expected. However, in glycogen-elicited peritoneal neutrophils, abundant soluble 5-lipoxygenase was in the nucleus. Upon activation with calcium ionophore A23187, intranuclear 5-lipoxygenase translocated to the nuclear envelope. Elicited neutrophils required a greater concentration of A23187 for activation than did blood neutrophils (half-maximal response, 160 versus 52 nM, respectively) but generated greater amounts of leukotriene B4 upon maximal stimulation (26.6 versus 7.68 ng/106 cells, respectively). Intranuclear 5-lipoxygenase was also evident in human blood neutrophils after adherence to a variety of surfaces, suggesting that adherence alone is sufficient to drive 5-lipoxygenase redistribution. These results demonstrate a physiologically relevant circumstance in which the subcellular distribution of 5-lipoxygenase can be rapidly altered in resting cells, independent of 5-lipoxygenase activation. Nuclear import of 5-lipoxygenase may be a universal accompaniment of neutrophil recruitment into sites of inflammation, and this may be associated with alterations in enzymatic function.
Leukotrienes (LTs)1 are potent lipid mediators derived from arachidonic acid (AA). They have important roles in regulating both normal cell functions, such as proliferation (1), and inflammatory processes implicated in disease states, such as asthma (2). The synthesis of LTs is initiated by the enzyme 5-lipoxygenase (5-LO) (3). Recent studies have demonstrated that the subcellular distribution of 5-LO differs among resting cells of different types: it is predominantly cytosolic in peripheral blood PMNs (4) and peritoneal macrophages (5), but it can be found in both the nucleus and cytosol of alveolar macrophages (6) as well as mast cells (7) and the mast cell-like rat basophilic leukemia cell line (4). Upon stimulation, both cytosolic and nuclear 5-LO can translocate to the nuclear envelope (6, 8, 9), where 5-LO can interact with the 5-lipoxygenase-activating protein (10) to oxygenate AA.
The LT synthetic capacity of a cell can be elevated via an increase in the amount of 5-LO (11, 12), 5-lipoxygenase-activating protein (13, 14), or phospholipase A2 (15, 16) protein. However, increases in LT synthetic capacity can also occur independent of changes in protein levels (17-19). This indicates that other mechanisms for increasing LT synthetic capacity must exist. The fact that 5-LO can exist in two distinct subcellular compartments (the cytoplasm and the nucleoplasm) raises the possibility that changes in 5-LO distribution may be subject to modulation. Such redistribution may, in turn, effect a change in LT synthetic capacity.
PMNs, purified from peripheral blood, are known to synthesize and secrete large amounts of LTB4 after stimulation. Blood PMNs are recruited rapidly and in large numbers into sites of inflammation and play a critical role in the rapid resolution of bacterial and fungal infections. Interestingly, PMNs recruited to sites of inflammation in rats have been found to produce even more LTB4 than blood PMNs (20). Because the recruitment of PMNs occurs rapidly, the enhanced LT synthetic capacity associated with recruitment may be expected to result from changes other than increases in 5-LO or 5-lipoxygenase-activating protein levels. In this study, we asked whether the recruitment of PMNs into sites of inflammation causes a change in the subcellular compartmentation of 5-LO protein.
Human PMNs were isolated from venous blood obtained from normal volunteers. Purification involved the sequential steps of centrifugation through Ficoll-Paque (Pharmacia Biotech, Inc.), dextran sedimentation, and hypotonic lysis of erythrocytes (21). Rat peripheral blood PMNs and elicited PMNs were from respiratory disease-free male Sprague Dawley retired breeder rats (Charles River Laboratories, Portage, MI). Rat peripheral blood PMNs were purified according to the human blood PMN purification protocol (purity, 90-97%).
Glycogen-elicited rat peritoneal leukocytes were obtained by standard methods (22). Briefly, 30 ml of 1.0% glycogen (Sigma) in saline were introduced into the peritoneum of diethyl ether-anesthetized rats; elicited leukocytes were recovered by peritoneal lavage, typically 4 h after glycogen instillation. Rat peritoneal leukocytes were also obtained 4 h after the introduction of heat-killed Cryptococcus neoformans (strain 52; American Type Culture Collection, Rockville, MD; 1 × 108 colony-forming unit equivalents in saline). Differential counts of cell populations from either procedure indicated that 85-95% of the cells were PMNs.
Bleomycin was used to induce inflammation in the lungs of rats by standard methods (23). Alveolar leukocytes were examined 2 days after intratracheal injection of bleomycin (0.75 unit/100 g body weight in 300 µl of saline). Leukocytes recovered by bronchoalveolar lavage (24) were processed for indirect immunofluorescent microscopy (see below). Alternatively, lung sections (from different animals) were processed for immunohistochemistry (see below). Human alveolar leukocytes were obtained from patients with pneumonia undergoing diagnostic bronchoalveolar lavage, as described (25). The experimental protocol was approved by the University of Michigan Medical Center Institutional Review Board for Approval of Research Involving Human Subjects.
Indirect Immunofluorescence Microscopy (IFM)Cells were
prepared for IFM as described previously (4), using methanol
(20 °C, 30 min) followed by acetone (
20 °C, 3 min) to fix and
permeabilize. They were then probed with a rabbit polyclonal antibody
raised against purified human leukocyte 5-LO (a generous gift of Dr. J. Evans, Merck Frosst Center for Therapeutic Research, Pointe
Claire-Dorval, Quebec, Canada; titer of 1:150) (8) followed by
rhodamine-conjugated goat anti-rabbit antibody (1:200; Sigma). In some
cases, cells were also stained for DNA using acridine orange (in the
presence of RNase). Preparations were examined with a Nikon Labophot 2 microscope equipped for epifluorescence or imaged by confocal
microscopy using a Bio-Rad MRC-600 laser confocal microscope. The
rhodamine signal was imaged using a 560-nm-long pass filter followed by
a 585-nm bandpass filter. Acridine orange fluorescence was isolated
using a 514-nm bandpass filter combined with a 526-nm-long pass
dichroic reflector.
As described previously (9), cells were disrupted by nitrogen cavitation at 400 p.s.i. for 5 min at 4 °C. Cavitate was centrifuged at 1000 × g to pellet nuclei; the postnuclear supernatant was centrifuged at 100,000 × g for 30 min at 4 °C to generate soluble ("cytosolic") and insoluble ("membrane") fractions. Nuclei were sonicated, and soluble and insoluble fractions were separated by ultracentrifugation. Equivalent amounts of protein from each fraction were evaluated by immunoblot (5) using 5-LO antibody (1:5000) and then peroxidase-conjugated goat anti-rabbit secondary (1:5000) with chemiluminescent detection (Amersham).
ImmunohistochemistryImmunohistochemistry, as described (26), utilized lung tissue specimens fixed in neutral-buffered formalin, embedded in paraffin, sliced, mounted, deparaffinized (Americlear), and rehydrated in descending concentrations of ethanol. Tissue was blocked (Power Block; Biogenics, San Ramon, CA), probed with 5-LO antibody (1:500, 4 °C, 24 h), washed, and then incubated with biotinylated goat anti-rabbit IgG (1:600). After washing, sections were incubated with avidin-conjugated horseradish peroxidase reagent for 45 min, washed, incubated with True-Blue peroxidase substrate (KPL Laboratories, Gaithersburg, MD), and then counterstained with Contrast Red (KPL Laboratories).
Cell Activation and Enzyme ImmunoassayPMNs in M199 at
106 cells/ml1 were activated with calcium
ionophore A23187. After 15 min at 37 °C, cells were pelleted, and the LTB4 concentration in the conditioned media was
determined by enzyme immunoassay (Cayman Chemical, Ann Arbor, MI).
Average values of duplicate determinations were obtained in each
experiment.
Statistical significance was evaluated by a paired Student's t test, using p < 0.05 as indicative of statistical significance.
The distribution of 5-LO was evaluated by two
complementary techniques: 1) IFM, and 2) cell fractionation combined
with immunoblotting. By IFM, 5-LO was predominantly cytosolic in PMNs
purified from peripheral blood (Fig. 1A), as
has been described for human blood PMNs (4). This pattern was observed
in essentially all blood PMNs. In sharp contrast, most PMNs elicited
into the peritoneum after glycogen instillation showed the opposite
pattern: the nucleus stained strongly positive for 5-LO, whereas the
cytosol had negligible staining (Fig. 1B). This pattern was
evident in approximately 80% of all PMNs obtained by peritoneal lavage
after elicitation. Other PMNs showed either predominantly cytosolic
5-LO or a mix of both cytosolic and nuclear staining (arrow,
Fig. 1B). Peritoneal macrophages, a minor contaminant, had
predominantly cytosolic 5-LO (data not shown), as reported previously
(5).
When rat peripheral blood PMNs were analyzed as a population by fractionation and immunoblotting, 5-LO was found to be entirely soluble and exclusively in the cytosol (Fig. 1C), consistent with conclusions based on IFM. By the same method, 5-LO in lavaged peritoneal cells was divided between the cytosolic and nuclear soluble fractions. Thus, two independent methods, one that evaluated individual cells and another that analyzed cell populations, indicated that 5-LO was exclusively in the cytosol of peripheral blood PMNs, whereas glycogen-elicited PMNs contained abundant nuclear 5-LO. The apparent differences in the amount of cytosolic 5-LO in elicited PMNs as judged by the two methods may be attributed to, on the one hand, an underestimation due to loss during permeabilization for IFM and, on the other hand, an overestimation due to unavoidable disruption of some nuclei combined with fractionation of a heterogeneous population (i.e. PMNs with nuclear 5-LO mixed with some peritoneal macrophages, as well as PMNs, with cytosolic 5-LO).
The localization of 5-LO in elicited PMNs was further evaluated by
optical sectioning of stained cells, using confocal microscopy (Fig.
2). An optical section through the nucleus of elicited
PMNs stained for both DNA (using acridine orange) and 5-LO revealed colocalization of DNA and 5-LO in most cells, although some cells retained cytosolic 5-LO (arrow, Fig. 2A). Serial
sections through cells stained only for 5-LO demonstrated that 5-LO was
dispersed homogenously throughout the intranuclear volume rather than
distributed peripherally near the nuclear envelope (Fig.
2B).
5-LO Distribution in Other Types of Elicited PMNs
PMNs can be
recruited into a variety of tissue sites in response to a number of
different signals. We were interested in determining if the nuclear
import of 5-LO was unique to glycogen-elicited peritoneal PMNs. 5-LO
was also intranuclear in PMNs recovered from the rat peritoneum 4 h after instillation of heat-killed C. neoformans (Fig.
3A), indicating that the result was not
glycogen-specific. 5-LO was also found to be intranuclear in PMNs
recruited into rat lung 2 days after intratracheal instillation of
bleomycin as determined by either IFM of cells recovered from lung by
lavage (Fig. 3B) or immunohistochemistry of lung sections
(Fig. 3C). The demonstration of intranuclear 5-LO in
elicited PMNs in situ (by immunohistochemistry) indicated
that the redistribution did not result from the lavage process or the
subsequent handling of PMNs. As an example of elicited PMNs from
humans, PMNs recovered by bronchoalveolar lavage of patients with
pneumonia also exhibited intranuclear 5-LO (Fig. 3D). These
results showed that 5-LO movement from the cytosol into the nucleus
could occur in PMNs recruited into different anatomic sites, in
response to different agents, and in humans as well as in rats.
The Effect of Subcellular Distribution on Function
How does
5-LO redistribution affect 5-LO function? One hallmark of 5-LO action
is its translocation to the nuclear envelope upon cell stimulation, a
process that colocalizes 5-LO with the AA-binding protein,
5-lipoxygenase-activating protein. As reported for human blood PMNs (8,
9), after stimulation, 5-LO in rat blood PMNs was found predominantly
at the periphery of the multilobed nuclei, apparently at the nuclear
envelope (Fig. 4A). The subcellular
distribution of 5-LO in elicited PMNs after activation was also
consistent with translocation to the nuclear envelope (Fig.
4B). However, the pattern of distribution was subtly
different from that seen in blood PMNs: in blood PMNs, the nuclear
lobes and connecting strands were clearly outlined with fluorescence, whereas in elicited PMNs, only portions of the nuclear lobes were labeled. These patterns would be consistent with translocation to
different membrane faces of the nuclear envelope, with cytosolic 5-LO
decorating the outer membrane, and intranuclear 5-LO binding to the
inner membrane. Finally, the distribution of 5-LO in activated elicited
PMNs was distinctly different from that in resting elicited PMNs (Fig.
1B), again indicating that 5-LO in resting elicited PMNs was
not simply associated with the nuclear envelope.
Elicited PMNs, like blood PMNs, generated little LTB4
without exogenous stimulation (7.3 ± 2.3 versus
12.9 ± 2.4 pg/106 cells, respectively;
p = 0.21; n = 3), indicating that
elicitation itself did not activate the 5-LO pathway. We hypothesized
that a consequence of the shift in 5-LO localization seen with
elicitation might be a change in the dose of ionophore required for LT
synthesis. Specifically, we reasoned that more ionophore would be
needed to cause an increase in nuclear calcium and thus activate
nuclear 5-LO than would be needed to have the same result within the
cytosol. Indeed, significantly more ionophore was needed to stimulate
LTB4 synthesis in elicited PMNs than in peripheral blood
PMNs (half-maximal stimulation at 160 ± 16 versus
52 ± 4.6 nM A23187, respectively; p = 0.0027; n = 4). However, maximal LT synthetic capacity
for elicited PMNs (26.6 ± 7.4 ng/106 cells at
407 ± 210 nM A23187) exceeded that for blood PMNs
(7.68 ± 0.84 ng/106 cells at 165 ± 78 nM A23187) significantly (p = 0.044;
n = 4). Dose-response curves from a representative
experiment are shown in Fig. 5. Thus, a greater level of
stimulation was needed to initiate LT synthesis in elicited PMNs, but
the maximal LT synthetic capacity of elicited PMNs significantly
surpassed that of blood PMNs.
Possible Role for Adherence in Redistribution of 5-LO
PMN
recruitment is a multistep process, but one prerequisite for
recruitment to all anatomic sites is the adherence of PMNs to the
endothelium. If adherence triggers the redistribution of 5-LO from the
cytosol to the nucleus of PMNs, then PMNs examined at earlier time
points after recruitment should also show intranuclear 5-LO. Indeed,
PMNs recovered by peritoneal lavage at either 1 or 2 h after
glycogen instillation (in separate animals) exhibited intranuclear 5-LO
(Fig. 6). This indicated that the nuclear import of 5-LO
occurred relatively early in recruitment, resulting from an early
event, such as adherence, and was not necessarily a function of
prolonged residence in the inflammatory site. Furthermore, because
elicited PMNs from both human and rat sources demonstrated intranuclear
5-LO (Fig. 3), it seemed likely that a common process, like adherence,
could cause the nuclear import of 5-LO in PMNs from either source.
As an initial evaluation of the role of adherence in 5-LO
redistribution in human PMNs, peripheral blood PMNs were purified and
examined before and after adherence to glass. By IFM, 5-LO was
cytosolic in freshly purified human blood PMNs maintained in suspension
in Teflon cups (Fig. 7A), as expected. After
adherence to glass for 1 h, 5-LO was predominantly intranuclear
(Fig. 7C). A shift of 5-LO into the nucleus was evident as
early as 15 min after adherence (Fig. 7B). Intranuclear
localization of 5-LO was also prominent in PMNs adhered for 1 h to
albumin-coated glass or plastic (data not shown). When adherent PMNs
were detached by trypsinization, fractionated, and analyzed by
immunoblotting, abundant 5-LO was associated with the nuclear soluble
fraction, whereas 5-LO was solely cytosolic in PMNs in suspension (Fig. 7C). Thus, adherence alone is sufficient to induce the
redistribution of 5-LO from the cytosol into the nucleus.
It is well established that upon activation, 5-LO undergoes rapid translocation to the nuclear envelope. However, the subcellular distribution of 5-LO in resting cells has previously been viewed as static, although it was known to vary among cell types (27). The principle finding of this study is that the distribution of 5-LO can be dynamic, even in the resting cell: unstimulated PMNs in the peripheral blood have none of the enzyme associated with the nucleus, whereas elicited or adherent PMNs have abundant 5-LO within the nucleus. It is important to distinguish between the import into the nucleoplasm seen here and the translocation to the nuclear envelope associated with activation. The former, unlike the latter, was not associated with LT synthesis.
This study also demonstrated several important aspects of the shift in 5-LO distribution: 1) this redistribution can be relatively rapid. 2) The redistribution of 5-LO into the nucleus is a general feature of PMN recruitment to sites of inflammation: it can occur during elicitation into different sites, in response to different agents, and in both rats and humans. 3) 5-LO within the nucleus, like 5-LO in the cytosol, will translocate to the nuclear envelope upon cell stimulation. 4) Elicited PMNs, with predominantly intranuclear 5-LO, can not only synthesize LTs but can generate significantly greater amounts of LTs than blood PMNs, which have exclusively cytosolic 5-LO. 5) Nuclear sequestration seems to buffer the 5-LO pathway from activation. 6) Adherence alone is sufficient to induce redistribution of 5-LO.
The actual trigger for import is not known. Although adherence seems to rapidly promote nuclear import, different types of cell surfaces, adhesion molecules, and extracellular matrices may have different effects on the import of 5-LO. These have not been examined here. Also, the mechanism of 5-LO import into the nucleus is not known. Large molecules require either a nuclear localization sequence or a chaperone with a nuclear localization sequence to traverse nuclear pores (28). The 5-LO protein has a region that is rich in basic amino acids (amino acids 650-657) that might serve as a nuclear localization sequence. Furthermore, the dynamic nature of 5-LO import suggests that mechanisms for regulating 5-LO redistribution must exist. Likely mechanisms include direct modification [e.g., phosphorylation, as has recently been described (29)] of the 5-LO protein itself or a change in an unidentified accessory molecule, such as an import-chaperone protein or a cytosolic tethering protein. These possibilities await clarification.
The functional importance of the 5-LO redistribution that we have described is unclear, but it could have ramifications for enzyme activation. 5-LO activation is calcium-dependent (30). In some cell types, changes in intranuclear calcium levels seem to be independent of changes in cytosolic calcium (31), whereas in other cell types, the two apparently are linked (32). Theoretically, an agonist that increased calcium exclusively in the cytosol would activate 5-LO (and initiate LT synthesis) in blood PMNs but not in elicited PMNs. In such a scenario, the sequestration of 5-LO within the nucleus would thereby serve to decrease the susceptibility of the enzyme to activation. Consistent with this possibility, our data using ionophore demonstrated that more agonist was needed to drive LT synthesis in elicited PMNs than in blood PMNs. A similar pattern exists among macrophages: the threshold for initiation of LT synthesis is higher in alveolar macrophages, which have intranuclear 5-LO (6), than in peritoneal macrophages (24), which have cytosolic 5-LO (5). However, once triggered, the level of LTB4 production by nuclear 5-LO in elicited PMNs greatly exceeds that produced by cytosolic 5-LO in blood PMNs. It is interesting that just as alveolar macrophages have a higher activation threshold than peritoneal macrophages, they also have a greater maximal LTB4 synthetic capacity (24). The identical patterns of 5-LO distribution and action in macrophages and PMNs suggest a causal relationship between changes in 5-LO localization and altered AA metabolism. Although the basis for the greater maximal LT synthetic capacity in elicited PMNs and alveolar macrophages is not known, these results underscore the importance of intranuclear 5-LO as an active pool in LT generation.
Within the activated cell, cytosolic 5-LO will move to the outer membrane of the nuclear envelope, whereas intranuclear 5-LO will move to the inner membrane. These sites of 5-LO action are spatially distinct, being separated by a lumen. The function of activated 5-LO may therefore be influenced by its topographic proximity to substrate and cofactors, as well as other enzymes that act either upstream or downstream from it. In this manner, the disparate distributions of 5-LO in resting and elicited PMNs would also be expected to have further ramifications on molecular aspects of enzyme action. Furthermore, the subcellular localization of these other elements may also be dynamic rather than static. For example, the "cytosolic" phospholipase A2 is indeed cytosolic in quiescent endothelial cells but becomes intranuclear when the same cells are growing rapidly (33). Thus, the element of dynamic redistribution adds a new level of complexity to the process of AA liberation and 5-LO action.
The changeable compartmentation of 5-LO suggests novel roles for 5-LO
products and also for 5-LO itself. The rapid redistribution of 5-LO may
serve to regulate the site of 5-LO enzymatic action. This would be
particularly interesting if 5-LO products acted at the immediate site
of synthesis. For example, if the products of cytosolic 5-LO affected
cytosolic processes (e.g., cytoskeletal functioning), and
the products of nuclear 5-LO affected nuclear processes
(e.g., transcription), then 5-LO compartmentation could be a
way to regulate cell function. Such localized effects could be achieved
by much lower concentrations of LTs than are needed for extracellular
release and paracrine action. These effects might be mediated by
soluble intracellular receptors like the peroxisome
proliferator-activated receptor , which can bind LTB4 in
the nucleus (34). Alternatively, the 5-LO protein itself has sites for
interacting with other proteins, including a Src homology 3-binding
domain (35). Such domains mediate the interaction of 5-LO with other
proteins (35), suggesting the possibility of function(s) for 5-LO
independent of its enzymatic activity. The rapid redistribution of
5-LO, then, could serve as a mechanism for regulating the accessibility
of 5-LO to other proteins and thus controlling such (hypothetical)
effects.
The potential for rapid movement of 5-LO between the cytosol and the nucleus in a single cell type, independent of activation, indicates a level of complexity in 5-LO action that has heretofore been unappreciated. Furthermore, this study correlates the import of 5-LO into the nucleus with an increase in cellular LT synthetic capacity. The molecular mechanisms of both 5-LO redistribution and altered LT synthetic capacity remain to be determined.