Neutrophil transit time and localization within the megakaryocyte define morphologically distinct forms of emperipolesis

AbstractIn emperipolesis, neutrophils transit through megakaryocytes, but it is unknown whether this interaction represents a single type of cell-in-cell interaction or a set of distinct processes. Using an in vitro model of murine emperipolesis, we characterized neutrophils entering megakaryocytes using live-cell spinning disk microscopy and electron microscopy. Approximately half of neutrophils exited the megakaryocyte rapidly, typically in 10 minutes or less, displaying ameboid morphology as they passed through the host cell (fast emperipolesis). The remaining neutrophils assumed a sessile morphology, most remaining within the megakaryocyte for at least 60 minutes (slow emperipolesis). These neutrophils typically localized near the megakaryocyte nucleus. By ultrastructural assessment, all internalized neutrophils remained morphologically intact. Most neutrophils resided within emperisomes, but some could be visualized exiting the emperisome into the cell cytoplasm. Neutrophils in the cytoplasm assumed close contact with the platelet-forming demarcation membrane system or with the perinuclear endoplasmic reticulum, as confirmed by immunofluorescence microscopy. Together, these findings reveal that megakaryocyte emperipolesis reflects at least two processes, fast and slow emperipolesis, each with its own characteristic transit time, morphology, and intracellular localization, suggesting distinct functions.Key PointsNeutrophil passage through megakaryocytes, termed emperipolesis, diverges into fast and slow forms that differ in transit time, morphology, and intracellular localizationDuring emperipolesis, neutrophils can reside in vacuoles (emperisomes) or escape into the cell cytoplasm to assume positions near the megakaryocyte’s demarcation membrane system, endoplasmic reticulum, or nucleus.

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Neutrophil transit time and localization within the megakaryocyte define morphologically distinct forms of emperipolesis

Blood Advances ◽

10.1182/bloodadvances.2021005097 ◽

2021 ◽

Author(s):

Frank Y. Huang ◽

Pierre Cunin ◽

Felix Andreas Radtke ◽

Roxane Darbousset ◽

Ricardo Grieshaber-Bouyer ◽

...

Keyword(s):

Transit Time ◽

In Vitro Model ◽

Close Contact ◽

Membrane System ◽

Cell Interaction ◽

Single Type ◽

Cell Cytoplasm ◽

Vitro Model ◽

In Transit

Neutrophils transit through megakaryocytes in a process termed emperipolesis, but it is unknown whether this interaction is a single type of cell-in-cell interaction or a set of distinct processes. Using a murine in vitro model, we characterized emperipolesis by live-cell spinning disk microscopy and electron microscopy. Approximately half of neutrophils exited the megakaryocyte rapidly, typically in 10 minutes or less, displaying ameboid morphology as they passed through the host cell (fast emperipolesis). The remaining neutrophils assumed a sessile morphology, most remaining within the megakaryocyte for at least 60 minutes (slow emperipolesis). These neutrophils typically localized near the megakaryocyte nucleus. By ultrastructural assessment, all internalized neutrophils remained morphologically intact. Most neutrophils resided within emperisomes, but some could be visualized exiting the emperisome to enter the cell cytoplasm. Neutrophils in the cytoplasm assumed close contact with the platelet-forming demarcation membrane system or the perinuclear endoplasmic reticulum. These findings reveal that megakaryocyte emperipolesis reflects at least two distinct processes differing in transit time and morphology, fast and slow emperipolesis, suggesting divergent physiologic functions.

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Secretion ofSaccharomyces cerevisiaeKiller Toxin: Processing of the Glycosylated Precursor

Molecular and Cellular Biology ◽

10.1128/mcb.3.8.1362 ◽

1983 ◽

Vol 3 (8) ◽

pp. 1362-1370 ◽

Cited By ~ 61

Author(s):

H. Bussey ◽

D. Saville ◽

D. Greene ◽

D. J. Tipper ◽

K. A. Bostian

Keyword(s):

Endoplasmic Reticulum ◽

Secretory Pathway ◽

Killer Toxin ◽

Membrane System ◽

Restrictive Temperature ◽

Wild Type ◽

Endoproteolytic Cleavage ◽

Toxin Secretion

Killer toxin secretion was blocked at the restrictive temperature inSaccharomyces cerevisiae secmutants with conditional defects in theS. cerevisiaesecretory pathway leading to accumulation of endoplasmic reticulum (sec18), Golgi (sec7), or secretory vesicles (sec1). A 43,000-molecular-weight (43K) glycosylated protoxin was found by pulse-labeling in allsecmutants at the restrictive temperature. Insec18the protoxin was stable after a chase; but insec7andsec1the protoxin was unstable, and insec111K toxin was detected in cell lysates. The chymotrypsin inhibitor tosyl-l-phenylalanyl chloromethyl ketone (TPCK) blocked toxin secretion in vivo in wild-type cells by inhibiting protoxin cleavage. The unstable protoxin in wild-type and insec7andsec1cells at the restrictive temperature was stabilized by TPCK, suggesting that the protoxin cleavage was post-sec18and was mediated by a TPCK-inhibitable protease. Protoxin glycosylation was inhibited by tunicamycin, and a 36K protoxin was detected in inhibited cells. This 36K protoxin was processed, but toxin secretion was reduced 10-fold. We examined twokexmutants defective in toxin secretion; both synthesized a 43K protoxin, which was stable inkex1but unstable inkex2. Protoxin stability inkex1 kex2double mutants indicated the orderkex1→kex2in the protoxin processing pathway. TPCK did not block protoxin instability inkex2mutants. This suggested that theKEX1- andKEX2-dependent steps preceded thesec7Golgi block. We attempted to localize the protoxin inS. cerevisiaecells. Use of an in vitro rabbit reticulocyte-dog pancreas microsomal membrane system indicated that protoxin synthesized in vitro could be inserted into and glycosylated by the microsomal membranes. This membrane-associated protoxin was protected from trypsin proteolysis. Pulse-chased cells or spheroplasts, with or without TPCK, failed to secrete protoxin. The protoxin may not be secreted into the lumen of the endoplasmic reticulum, but may remain membrane associated and may require endoproteolytic cleavage for toxin secretion.

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Megakaryocyte emperipolesis mediates membrane transfer from intracytoplasmic neutrophils to platelets

eLife ◽

10.7554/elife.44031 ◽

2019 ◽

Vol 8 ◽

Cited By ~ 16

Author(s):

Pierre Cunin ◽

Rim Bouslama ◽

Kellie R Machlus ◽

Marta Martínez-Bonet ◽

Pui Y Lee ◽

...

Keyword(s):

Bone Marrow ◽

Dynamic Process ◽

Membrane System ◽

Cell Interaction ◽

Platelet Production ◽

Β2 Integrin ◽

Membrane Bound ◽

Membrane Transfer

Bone marrow megakaryocytes engulf neutrophils in a phenomenon termed emperipolesis. We show here that emperipolesis is a dynamic process mediated actively by both lineages, in part through the β2-integrin/ICAM-1/ezrin pathway. Tethered neutrophils enter in membrane-bound vesicles before penetrating into the megakaryocyte cytoplasm. Intracytoplasmic neutrophils develop membrane contiguity with the demarcation membrane system, thereby transferring membrane to the megakaryocyte and to daughter platelets. This phenomenon occurs in otherwise unmanipulated murine marrow in vivo, resulting in circulating platelets that bear membrane from non-megakaryocytic hematopoietic donors. Transit through megakaryocytes can be completed as rapidly as minutes, after which neutrophils egress intact. Emperipolesis is amplified in models of murine inflammation associated with platelet overproduction, contributing to platelet production in vitro and in vivo. These findings identify emperipolesis as a new cell-in-cell interaction that enables neutrophils and potentially other cells passing through the megakaryocyte cytoplasm to modulate the production and membrane content of platelets.

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Metabolism and intracellular localization of a fluorescently labeled intermediate in lipid biosynthesis within cultured fibroblasts.

The Journal of Cell Biology ◽

10.1083/jcb.91.3.872 ◽

1981 ◽

Vol 91 (3) ◽

pp. 872-877 ◽

Cited By ~ 54

Author(s):

R E Pagano ◽

K J Longmuir ◽

O C Martin ◽

D K Struck

Keyword(s):

Endoplasmic Reticulum ◽

Phosphatidic Acid ◽

Cultured Cells ◽

Large Fraction ◽

Intracellular Localization ◽

Chinese Hamster ◽

Cultured Fibroblasts ◽

Acid Analogue ◽

Unique Method

In this paper we report on the uptake and distribution of an exogenously supplied fluorescent phosphatidic acid analogue by Chinese hamster fibroblasts. Under appropriate in vitro incubation conditions, 1-acyl-2-(N-4-nitrobenzo-2-oxa-1,3-diazole)-aminocaproyl phosphatidic acid was rapidly and preferentially transferred from phospholipid vesicles to cells at 2 degrees C. However, unlike similar fluorescent derivatives of phosphatidylcholine and phosphatidylethanolamine that remain restricted to the plasma membrane under such incubation conditions (Struck, D. K., and R. E. Pagano. 1080. J. Biol. Chem. 255:5405--5410), most of the phosphatidic acid-derived fluorescence was localized at the nuclear membrane, endoplasmic reticulum, and mitochondria. This was shown by labeling cells with rhodamine-containing probes specific for mitochondria or endoplasmic reticulum, and comparing the patterns of intracellular NBD and rhodamine fluorescence. Extraction and analysis of the fluorescent lipids associated with the cells after treatment with vesicles at 2 degrees or 37 degrees C revealed that a large fraction of the fluorescent phosphatidic acid was converted to fluorescent diglyceride, phosphatidylcholine, and triglyceride. Our findings suggest that fluorescent phosphatidic acid may be useful in correlating biochemical studies of lipid metabolism in cultured cells and studies of the Intracellular localization of the metabolites by fluorescence microscopy. In addition, this compound provides a unique method for visualizing the endoplasmic reticulum in living cells.

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Examining rhodopsin retention in endoplasmic reticulum and intracellular localization in vitro and in vivo by using truncated rhodopsin fragments

Journal of Cellular Biochemistry ◽

10.1002/jcb.22942 ◽

2011 ◽

Vol 112 (2) ◽

pp. 520-530 ◽

Cited By ~ 3

Author(s):

Yuh-Fang Chen ◽

I-Jong Wang ◽

Luke L.K. Lin ◽

Muh-Shy Chen

Keyword(s):

Endoplasmic Reticulum ◽

Intracellular Localization

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A Human Sequence Homologue of Staufen Is an RNA-Binding Protein That Is Associated with Polysomes and Localizes to the Rough Endoplasmic Reticulum

Molecular and Cellular Biology ◽

10.1128/mcb.19.3.2212 ◽

1999 ◽

Vol 19 (3) ◽

pp. 2212-2219 ◽

Cited By ~ 115

Author(s):

Rosa María Marión ◽

Puri Fortes ◽

Ana Beloso ◽

Carlos Dotti ◽

Juan Ortín

Keyword(s):

Endoplasmic Reticulum ◽

Rough Endoplasmic Reticulum ◽

Rna Binding ◽

Intracellular Localization ◽

Binding Activity ◽

Ns1 Protein ◽

Binding Domains ◽

Human Sequence ◽

Dsrna Binding

ABSTRACT In the course of a two-hybrid screen with the NS1 protein of influenza virus, a human clone capable of coding for a protein with high homology to the Staufen protein from Drosophila melanogaster (dmStaufen) was identified. With these sequences used as a probe, cDNAs were isolated from a λ cDNA library. The encoded protein (hStaufen-like) contained four double-stranded RNA (dsRNA)-binding domains with 55% similarity and 38% identity to those of dmStaufen, including identity at all residues involved in RNA binding. A recombinant protein containing all dsRNA-binding domains was expressed in Escherichia coli as a His-tagged polypeptide. It showed dsRNA binding activity in vitro, with an apparentKd of 10−9 M. Using a specific antibody, we detected in human cells a major form of the hStaufen-like protein with an apparent molecular mass of 60 to 65 kDa. The intracellular localization of hStaufen-like protein was investigated by immunofluorescence using a series of markers for the cell compartments. Colocalization was observed with the rough endoplasmic reticulum but not with endosomes, cytoskeleton, or Golgi apparatus. Furthermore, sedimentation analyses indicated that hStaufen-like protein associates with polysomes. These results are discussed in relation to the possible functions of the protein.

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Nuclear pore complex integrity requires Lnp1, a regulator of cortical endoplasmic reticulum

Molecular Biology of the Cell ◽

10.1091/mbc.e15-01-0053 ◽

2015 ◽

Vol 26 (15) ◽

pp. 2833-2844 ◽

Cited By ~ 26

Author(s):

Amanda K. Casey ◽

Shuliang Chen ◽

Peter Novick ◽

Susan Ferro-Novick ◽

Susan R. Wente

Keyword(s):

Endoplasmic Reticulum ◽

Nuclear Pore Complex ◽

Membrane System ◽

Nuclear Pore ◽

Cellular Functions ◽

Genes Encoding ◽

Assembly Factor ◽

And Function ◽

Cortical Endoplasmic Reticulum

The nuclear envelope (NE) and endoplasmic reticulum (ER) are components of the same contiguous membrane system and yet have distinct cellular functions. Mounting evidence suggests roles for some ER proteins in the NE for proper nuclear pore complex (NPC) structure and function. In this study, we identify a NE role in Saccharomyces cerevisiae for Lnp1 and Sey1, proteins required for proper cortical ER formation. Both lnp1Δ and sey1Δ mutants exhibit synthetic genetic interactions with mutants in genes encoding key NPC structural components. Both Lnp1 and Sey1 physically associate with other ER components that have established NPC roles, including Rtn1, Yop1, Pom33, and Per33. Of interest, lnp1Δ rtn1Δ mutants but not rtn1Δ sey1Δ mutants exhibit defects in NPC distribution. Furthermore, the essential NPC assembly factor Ndc1 has altered interactions in the absence of Sey1. Lnp1 dimerizes in vitro via its C-terminal zinc finger motif, a property that is required for proper ER structure but not NPC integrity. These findings suggest that Lnp1's role in NPC integrity is separable from functions in the ER and is linked to Ndc1 and Rtn1 interactions.

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Megakaryocyte emperipolesis mediates membrane transfer from intracytoplasmic neutrophils to platelets

10.1101/504555 ◽

2018 ◽

Cited By ~ 1

Author(s):

Pierre Cunin ◽

Rim Bouslama ◽

Kellie R. Machlus ◽

Marta Martínez-Bonet ◽

Pui Y. Lee ◽

...

Keyword(s):

Bone Marrow ◽

Dynamic Process ◽

Membrane System ◽

Cell Interaction ◽

Platelet Production ◽

Β2 Integrin ◽

Membrane Bound ◽

Membrane Transfer

SummaryBone marrow megakaryocytes engulf neutrophils in a phenomenon termed emperipolesis. We show here that emperipolesis is a dynamic process mediated actively by both lineages, in part through the β2-integrin/ICAM-1/ezrin pathway. Tethered neutrophils enter in membrane-bound vesicles before penetrating into the megakaryocyte cytoplasm. Intracytoplasmic neutrophils develop membrane contiguity with the demarcation membrane system, thereby transferring membrane to the megakaryocyte and to daughter platelets. This phenomenon occurs in otherwise unmanipulated marrowin vivo, resulting in circulating platelets that bear membrane from non-megakaryocytic hematopoietic donors. Transit through megakaryocytes can be completed as rapidly as minutes, after which neutrophils egress intact. Emperipolesis is amplified in models of inflammation associated with platelet overproduction, contributing to platelet productionin vitroandin vivo.These findings identify emperipolesis as a new cell-in-cell interaction that enables neutrophils and potentially other cells passing through the megakaryocyte cytoplasm to modulate the production and membrane content of platelets.

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In Vitro Induction of Crystals of MT Protein by Vinblastine-Colcemid in Mouse Spermatids

Proceedings, annual meeting, Electron Microscopy Society of America ◽

10.1017/s0424820100050676 ◽

1974 ◽

Vol 32 ◽

pp. 132-133

Author(s):

John J. Wolosewick ◽

John H. D. Bryan

Keyword(s):

Endoplasmic Reticulum ◽

Smooth Endoplasmic Reticulum ◽

Nuclear Ring ◽

Rough Er ◽

Distal Direction ◽

In Vitro Induction

Early in spermiogenesis the manchette is rapidly assembled in a distal direction from the nuclear-ring-densities. The association of vesicles of smooth endoplasmic reticulum (SER) and the manchette microtubules (MTS) has been reported. In the mouse, osmophilic densities at the distal ends of the manchette are the organizing centers (MTOCS), and are associated with the SER. Rapid MT assembly and the lack of rough ER suggests that there is an existing pool of MT protein. Colcemid potentiates the reaction of vinblastine with tubulin and was used in this investigation to detect this protein.

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Modification of Pineal Ultrastructure by Exogenous Hormones

Proceedings, annual meeting, Electron Microscopy Society of America ◽

10.1017/s0424820100060866 ◽

1967 ◽

Vol 25 ◽

pp. 170-171

Author(s):

R. A. Turner ◽

A. E. Rodin ◽

D. K. Roberts

Keyword(s):

Electron Microscopy ◽

Endoplasmic Reticulum ◽

Rough Endoplasmic Reticulum ◽

Estradiol Benzoate ◽

Female Rats ◽

List Type ◽

Type Number ◽

Pregnant Rats ◽

Gonadal Atrophy ◽

Pineal Ultrastructure

There have been many reports which establish a relationship between the pineal and sexual structures, including gonadal hypertrophy after pinealectomy, and gonadal atrophy after injection of pineal homogenates or of melatonin. In order to further delineate this relationship the pineals from 5 groups of female rats were studied by electron microscopy:ControlsPregnant ratsAfter 4 weekly injections of 0.1 mg. estradiol benzoate.After 8 daily injections of 150 mcgm. melatonin (pineal hormone).After 8 daily injections of 3 mg. serotonin (melatonin precursor).No ultrastructural differences were evident between the control, and the pregnancy and melatonin groups. However, the estradiol injected animals exhibited a marked increase in the amount and size of rough endoplasmic reticulum within the pineal cells.

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