ABSTRACT
Intracellular pathogens are challenged with limited space and resources while replicating in a single host cell. Mechanisms for direct invasion of neighboring host cells have been discovered in cell culture, but we lack an understanding of how bacteria directly spread from cell-to-cell in vivo. Here, we describe the discovery of a bacterial species that uses filamentation as an in vivo mechanism for intracellular spreading between the intestinal epithelial cells of its host, the rhabditid nematode Oscheius tipulae. In vitro and in vivo filamentation by this bacterium, Bordetella atropi, requires a highly conserved nutrient-sensing pathway used by divergent bacteria to detect rich conditions and inhibit the divisome. Thus, B. atropi uses a distinct mechanism for cell-to-cell spreading by coopting a pathway that normally regulates bacterial cell size to trigger filamentation inside host cells.
INTRODUCTION
Pathogenic invasion of host cells often provides microbes with a major benefit, including a high concentration of metabolic resources and protection from extracellular immunity1. An individual host cell, however, represents a small niche and it is advantageous for intracellular pathogens to spread to other cells in order to maximize the use of host resources. All intracellular microbes can spread via extracellular escape from the initial infected cell, a process that leaves them vulnerable to host defenses. Some microbes, however, have evolved unique mechanisms to invade uninfected host cells directly from an initial infected cell. To date, two main paradigms for cell-to-cell spreading by bacteria have been described, both of which converge on effector-driven manipulation of host actin. In one mechanism, Listeria monocytogenes, Shigella flexneri, and Rickettsia spp. can polymerize host actin for cytoplasmic propulsion of bacteria into the lateral membrane for uptake by neighboring cells2. Burkholderia spp. also use actin-based propulsion, but invasion of neighboring cells is facilitated by fusion of the lateral membranes3. In another mechanism, Ehrlichia chaffeensis can directly transfer from a phagocytic cell to a target cell through actin-dependent filopodia formation, although it is unclear if this mechanism is directly initiated by the pathogen1,4. Each of these bacterial mechanisms has only been directly observed in cell culture systems, bringing up the possibility of alternative mechanisms for cell-to-cell spreading and dissemination in vivo5.
Bacteria often change their cell shape as a fitness strategy to survive or thrive in diverse environments. Filamentation is an example of this morphological plasticity, often used as a survival strategy in toxic or stressful environments. During filamentation, there is a dramatic increase in cell length as a bacterium divides longitudinally multiple times without daughter cell separation, often without septation6,7. Gram-negative bacteria are mainly known to undergo filamentation after exposure to environmental stressors, including DNA damage and β-lactam antibiotics, which induce the SOS response6. Several bacterial pathogens, such as H. influenzae, P. aeruginosa, Y. pestis, have been observed to filament in vivo, including inside host cells8. However, to our knowledge, filamentation has never been observed to be used for cell-to-cell spreading by any intracellular pathogen, including bacteria or fungi9. In this work, we describe the discovery of an intracellular bacterial pathogen that uses filamentation to directly spread from cell to cell in the intestine of an animal host. Initiation of intracellular filamentation by this pathogen requires a highly conserved metabolic pathway used by divergent bacteria to detect rich conditions to delay divisome assembly.
RESULTS
Discovery and characterization of Bordetella atropi
Wild-caught nematodes and their naturally associated pathogens have served as models to dissect different aspects of host-microbe interactions10–12. Given their transparency, these nematodes allow for the visualization and dissection of novel aspects of microbial pathogenesis and host immune/stress responses13–15. Known natural intracellular pathogens infecting free-living nematodes include viruses and microsporidia, but prior to now, no intracellular bacteria have been identified16. From ecological sampling, we isolated a wild Oscheius tipulae strain (JU1501) from rotting crab apples (Supplementary Fig. 1). O. tipulae is a rhabditid species that is commonly found in soil and decomposing vegetation17. In JU1501, coccobacilli-shaped microbes were observed to infect the intestinal epithelial cells (Fig. 1a). Since microsporidian parasites are the most common intracellular pathogens found in wild C. elegans and other free-living nematodes18,19, this microbe was originally reported in a large survey of microsporidia based on morphology, despite the failure of microsporidian-specific 18S primers to produce an amplicon19. We conducted fluorescence in situ hybridization (FISH) on mixed-stage populations of this O. tipulae strain and found that a mixture of microsporidian-specific 18S probes failed to bind (Supplementary Fig. 2a). Given the lack of hybridization of this microbe to commonly infecting microsporidian species associated with wild nematodes, we suspected it may instead be a bacterium. Indeed, a universal probe to bacterial 16S rRNA showed strong hybridization with a multitude of coccobacilli inside the animals (Fig. 1b). In addition to these coccobacilli, we also observed a second bacterial morphology in some animals in the same sample in which long filaments extended throughout the intestine (Fig. 1c). Identical phenotypes were seen using a FISH probe specific to the 16S rRNA of this filamenting coccobacillus bacterium but not a non-specific bacterial 16S probe (Supplementary Fig. 2b-c).
We isolated this bacterium on LB agar plates (strain name LUAb4) and verified that it could reinfect JU1501 O. tipulae animals that were sterilized of all horizontally-transmitted microbes using a bleach treatment (as seen Fig. 1e-g). We sequenced the genome of LUAb4 and conducted phylogenomic analysis to find that the bacterium represents a new species in a separate monophyletic clade of Bordetella (Fig. 1d), clustering with Bordetellae isolated from human respiratory specimens or the environment. We named this bacterium Bordetella atropi, after Atropos, the Greek Fate who cuts the thread of life (Supp. Text 1, Taxonomic Summary). Similar to other Bordetellae, B. atropi has the appearance of a coccobacillus morphology when in its non-filamentous form20. Infection by B. atropi has a severe effect on host fitness with an approximate 2.5-fold decrease in average lifespan and 90-fold decrease in fecundity (Fig. 1e-f). To determine the order of appearance of B. atropi phenotypes in vivo, we conducted a pulse-chase infection experiment and found that the most animals had a majority of bacteria displaying either short or long intracellular filaments at 16 and 24 hours post infection (hpi), while most animals had a majority of bacteria in the coccobacilli form at 38 and 48 hpi (Fig. 1g). When we used confocal microscopy on FISH-stained animals at 34 hours post infection (hpi), we found that the average in vivo filament length of WT B. atropi was 51.9 μm with a maximum of 130 μm, or approximately 130 bacterial cell lengths (Fig. 1h).
Bordetella atropi is an intestinal intracellular pathogen
Our observations of B. atropi infection by light microscopy suggested that coccobacilli were predominantly inside intestinal epithelial cells (Fig. 1a). To verify the intracellular nature and tissue tropism of B. atropi, we conducted transmission electron microscopy (TEM) of infected animals at 24 and 48 hpi. The intestine of O. tipulae is comprised of pairs of tubulating epithelial cells along the anterior-posterior axis, except at the most anterior portion of the intestine where four epithelial cells surround the lumen21. This intestine is separated from the body wall muscle, epidermis, and germline by a narrow space that forms the pseudocoelom (Fig. 2a). In uninfected animals, the intestinal cells can be distinguished by a relatively lighter electron density than other tissues, the presence of the intestinal lumen with microvilli, and a uniform distribution of intracellular gut granules (Fig. 2b). B. atropi coccobacilli and filaments were distinguished from host cellular structures by a wavy, electron dense cell wall surrounding large, electron poor nucleoids, similar to TEM images of intracellular Bordetella bronchiseptica22, and these phenotypes were not observed in uninfected animals (Fig. 2c-e). At 24 hpi, we can see filaments with this characteristic cell wall delineation in intestinal cells that are unseptated with regularly spaced nucleoids and coccobacilli in the intestinal lumen (Fig. 2f-g). TEM only captures a portion of a filament length due to thin sectioning and the longest filament captured with this method was 10.06 μm (Fig. 2f), as compared to the average filament length of 51.86 μm as determined by tracing individual distinguishable filaments by confocal microscopy (see Fig. 1h). Of note, we also observed instances where nucleoids appear to be dividing and potential septum formation in these filaments (Fig. 2g). By 48 hpi, we see intestinal cells that are heavily infected with individual coccobacilli cells (Fig. 2h). Notably, in cases where we could see lumenal bacteria at both 24 hpi and 48 hpi time points, the lumenal coccobacilli bear the same morphological characteristics of those detected in the intracellular environment (see Fig. 2c, lower right for lumenal coccobacilli). Using quantification, we found that 42% of images displayed intestinal filaments at 24 hpi (n=52), and only 6.5% at 48 hpi (n=31), showing a similar trend to the emergence of phenotypes in vivo via fluorescence microscopy (see Fig. 1g). Separately, TEM bolstered the intestinal tropism seen with B. atropi as 70.6% of images had intracellular intestinal infection (n=102), but no infection was seen in non-intestinal tissues, including the muscle (n=38) and epidermis (n=73). The lateral intestinal membranes appear disrupted in infected animals as they are often missing or at oblique angles relative to the intestinal lumen in infected cells. This is in contrast to uninfected cells where they are relatively perpendicular to the lumen (Supplementary Fig. 3). While the use of electron dense delineation cannot unambiguously identify B. atropi, their absence in uninfected animals, the morphological similarities between those seen in intestinal cells and the lumen, as well as their high abundance at 48 hpi (similar to the FISH time course) indicate that these structures are characteristic of B. atropi. Together, these observations suggest that B. atropi is an intracellular pathogen that first filaments in intestinal epithelial cells and later septates into individual coccobacilli before exiting the host cell.
As a parallel approach to TEM, we also employed fluorescent dyes that mark the intracellular environment of intestinal cells and confocal microscopy to investigate the localization of B. atropi in infected animals. Using CFSE, which strongly stains the cytoplasm of intestinal cells, we could observe the localization of B. atropi only within the boundary of the intestinal cell cytoplasm through z-stacks and orthogonal projections (Fig. 3a-b). Notably, we observed areas of CFSE-fluorescence clearing that overlap with the red fluorescence of B. atropi 16S probe (Fig. 3c, arrowheads in CFSE channel). This loss of CFSE fluorescence in these areas are likely due to bacterial filaments occupying these spaces, strongly supporting the cytoplasmic localization of B. atropi filaments (Fig. 3c).
Additionally, we used fluorophore-tagged phalloidin to stain host actin filaments, including apical ACT-5 and cortical actin filaments at the basolateral side of the intestine (Fig. 3d-e). In cases where phalloidin staining clearly showed the apical and basolateral perimeters of intestinal cells, we observed that B. atropi filaments and coccobacilli were localized within this actin staining. A representative line profile analysis shows that RFP-tagged bacteria lie in between positions of basal and apical actin filaments in the intestine and close to nucleus, suggesting that B. atropi localizes within intestinal cells (Fig. 3f). We quantitated these images and found that 92.5% of infection events (i.e., coccobacilli or filaments) stay well within the boundaries of intestinal actin filaments, whereas 7.5% of infection events were ambiguous in their localization as there was direct overlap with the basal actin filament and we could not clearly assign localization to them (Fig. 3g). However, we did not observe any infection events that were clearly extracellular, where bacterial phenotypes appeared beyond the basal actin filament boundary of intestinal cells (0% extracellular) nor did we observe bacteria colocalizing with the body wall muscle. Separately, with phalloidin straining we also observed instances where bacterial filaments were pushing through the lateral actin filaments of intestinal cells, suggesting that these filaments were crossing through the cell-cell boundary between intestinal cells, reminiscent of the TEM result (Fig. 3h-i). Altogether, these data strongly support the intracellular nature and intestinal tropism of B. atropi.
Filamentation by B. atropi is used for cell-to-cell spreading
We hypothesized that filamentation by B. atropi is used as a mechanism for cell-to-cell spreading. Often, we observed cases where filaments passed near multiple intestinal nuclei, indicating that the bacterium was simultaneously infecting neighboring intestinal cells (Fig. 4a). To test this hypothesis, we sought to isolate a non-filamenting mutant of B. atropi. Similar to Bordetella avium23, our bacterium could be induced to filament in vitro by switching growth from Luria broth (LB) to the richer medium Terrific broth (TB) (Supplementary Fig. 4a), allowing us to use in vitro selection to isolate filamentation mutants (Fig. 4b). We focused on one mutant, LUAb7, which formed less frequent and much shorter filaments in vitro compared to wild type (Fig. 4c) but grew at the same rate (Fig. 4d). In vivo infection of O. tipulae found that LUAb7 also showed significantly decreased anterior-posterior spreading (Supplementary Fig. 4b-c). We confirmed that LUAb7 still infects the cytoplasm of intestinal cells in vivo using the cytoplasmic dye CFSE (Supplementary Fig. 5a-b).
Further in vivo characterization of LUAb7 showed that the main phenotype of the bacteria in infected animals is coccobacilli throughout the course of infection, with areas filled with coccobacilli increasing as the infection progresses (Supplementary Fig. 5c-d). LUAb7 also forms much shorter filaments compared to WT, with an average length of 6.55 μm (Supplementary Fig. 5e), and even though LUAb7 failed to form long filaments in vivo, it still sufficiently reduced host genetic fitness to the same level as WT, suggesting that other virulence mechanisms may affect host fitness (Supplementary Fig. 5f-g).
The intestine of O. tipulae consists of left-right pairs of polarized epithelial cells running along the anterior-posterior (A-P) axis21 (Fig. 2a). To quantify the cell-to-cell spreading capacity of WT and LUAb7, we pulse infected animals for a short period to limit the number of invasion events and then counted the number of intestinal nuclei that each contiguous infection event passes along the A-P axis. A contiguous infection event is assumed to be the result of replication from a single bacterium. For distinguishable filaments, we assume each filament is the replicative product from a single invasion event. However, we also observed infection foci, especially with LUAb7 infection. These foci are tightly packed clusters of coccobacilli, or a mixture of closely spaced short filaments (4-8 μm) and coccobacilli, and each focus is well separated from each other (Supplementary Fig. 6). We assume one infection focus is the result of one infection event in which the original invading bacterium underwent normal binary division, however, it is also possible that an infection focus is the result of more than one infection event. We observed both phenotypes in animals infected with either WT or LUAb7 strain, albeit at markedly different frequencies. For the WT strain, 95% of infection events were filaments and 5% were foci (n=162), whereas 9% of infection events were distinguishable filaments (8-14 μm) and 91% were foci (n=131) in case of LUAb7. When we followed single WT B. atropi filaments in vivo, they spanned an average of 5.7 and a maximum of 15 intestinal nuclei (Fig. 4e-f). By contrast, LUAb7 failed to consistently form filaments in vivo, with replicating infection foci seen spanning an average of 1.9 and a maximum of 4 intestinal nuclei. Similar to C. elegans, intestinal nuclei in O. tipulae may undergo one nuclear division without cell division during development. Using intestinal membrane staining, we quantified an average of 1.9 intestinal nuclei per cell at both the anterior and posterior end (Supplementary Fig. 7). Therefore, WT B. atropi filaments spread laterally to an average of 3 cells and a maximum of 8 cells at 34 hpi, while the filamentation mutant remains largely restricted to a single cell but occasionally spreads to another cell. Altogether, these data indicate that B. atropi uses filamentation as an intracellular mechanism for cell-to-cell spreading.
A conserved metabolic pathway controls B. atropi filamentation
We identified the causative mutation in LUAb7 through whole genome sequencing and single nucleotide variations (SNVs) calling. The best candidate was a missense mutation found in gtaB, a UTP--glucose-1-phosphate uridylyltransferase. The mutation in gtaB lead to an R17C change in a predicted catalytic arginine found in a highly conserved N-terminal motif (Fig. 5a)24. We complemented LUAb7 with gtaB+ from B. atropi and found a rescue of in vitro filamentation (Fig. 5b) as well as in vivo filamentation, with similar levels of cell-to-cell spreading as wild type (Fig. 4e-f). Additionally, deletion of gtaB from WT B. atropi resulted in a loss of filamentation in vitro, similar to gtaBR17C (Fig. 5d). Thus, gtaBR17C is the causative allele for loss of filamentation in LUAb7 and this single mutation abolishes cell-to-cell spreading of the pathogen.
GtaB (GalU in E. coli) catalyzes the conversion of glucose-1-phosphate to UDP-glucose, a substrate in the production of cell wall components like osmoregulated periplasmic glucans (OPGs), lipopolysaccharide, and capsular polysaccharides (Fig. 4c). In E. coli and Bacillus subtilis, this UDP-glucose biosynthetic pathway serves as a metabolic sensor that links carbon availability to growth rate25. Excess UDP-glucose acts as a readout for rich conditions and temporarily inhibits FtsZ ring formation during replication for moderately larger progeny cells26,27. In E. coli, FtsZ ring inhibition is mediated by OpgH, a downstream glucosyltransferase that is thought to sequester FtsZ monomers at the nascent division site in a UDP-glucose-dependent manner (Fig. 5c)26. We tested other members in this pathway for a role in filamentation by knocking them out in B. atropi. Deletion of opgH resulted in a loss of filamentation in vitro, similar to LUAb7(gtaBR17C) (Fig. 5d). The B. atropi genomes contained two copies of phosphoglucomutase (pgm) and deletion of pgm2 but not pgm1 resulted in loss of in vitro filamentation (Fig. 5d). Surprisingly, knockout of pgm1 did not phenocopy LUAb7 but instead led to an increase in in vitro filamentation. This finding suggests that pgm1 may negatively regulate UDP-glucose biosynthesis, as a similar role has been suggested for galF in E. coli, which may antagonize galU in the same pathway28.
We then tested these knockouts in vivo. The opgH knockout phenocopied LUAb7(gtaBR17C), with reduced A-P spreading in the intestine (Fig. 5e). We verified that this decreased A-P spreading was not due to decreased infectivity, as LUAb7 (gtaBR17C), ΔgtaB, and Δpgm1 all had similar initial invasion events as WT at 16 hpi under our pulse-chase infection procedure (Supplementary Fig. 8). By contrast, the pgm1 knockout showed no change in spreading in vivo compared to WT, consistent with in vitro data. While both the Δpgm2 and ΔgtaB strains showed an inability to filament in vitro, we found that they were attenuated in vivo, as we saw no intracellular infection with these strains despite populations of >500 animals per replicate (Supplementary Fig. 9). In fact, we saw little to no bacteria in the intestinal lumen with these knockouts, suggesting that a complete loss of some cell wall components may result in an inability to survive feeding by O. tipulae, perhaps leaving bacteria sensitive to the posterior grinder and/or destruction by extracellular defenses in the lumen. Altogether, these results support a requirement for the UDP-glucose biosynthetic pathway and opgH in inhibiting cell fission in B. atropi, but in a more extreme manner than seen in E. coli and B. subtilis, leading to long multinucleoid filaments rather than bacilli with modestly increased lengths. Overall, we propose a model where B. atropi detects the nutrient-rich intracellular environment of an intestinal cell through the UDP-glucose biosynthetic pathway and OpgH in order to initiate filamentation for cell-to-cell spreading (Fig. 5f).
DISCUSSION
Together, our findings describe bacterial filamentation as an in vivo mechanism for cell-to-cell spreading in a host epithelium. Several human-infecting bacterial pathogens have been observed to filament in vivo, including some that filament intracellularly, bringing up the possibility that some pathogens may use filamentation as a spreading mechanism7,8. Uropathogenic E. coli (UPEC) can form extremely long filaments inside umbrella cells, with conflicting data on whether these filaments are refractory to phagocytosis by macrophages after their release from host cells29,30. Intracellular bacterial filaments can distort host cell shape in cell culture, as Yersinia pestis filaments in macrophages can make protrusions in the host cell membrane31 and Salmonella typhimurium filaments can grossly distort and elongate primary melanocytes32. We observed similar phenotype in B. atropi whereby bacterial filaments push against and distort the lateral actin filaments of host intestinal cells. It is possible that exaggerated longitudinal growth is an in vivo strategy that intracellular pathogens can use to push through the lateral membranes in an epithelial layer for invasion of neighboring cells. For example, microsporidian parasites in C. elegans can form elongated intracellular stages (called meronts) that distort lateral intestinal membranes, leading to the formation of a syncytial tissue and cell-cell spreading13.
We found that filamentation induction by B. atropi is linked to nutrient availability through a highly conserved metabolic pathway that inhibits the bacterial divisome under rich conditions. These findings represent a new mechanism for the induction of filamentation in bacteria that is independent of the SOS response. Given the broad conservation of the UDP-glucose pathway and its role in delaying binary division on rich media26,27, it is possible that the evolutionary steps for coopting this pathway for filamentation are minimal. For example, experimental overexpression of opgH in E. coli is sufficient to lead to filamentation, showing that altering the expression of a single gene in the pathway can induce this phenotype26. B. avium is a respiratory pathogen of turkeys and was found to form filaments in TB similar to B. atropi, bringing up the possibility that filamentation in rich conditions is conserved among other clinically-relevant Bordetellae23.
METHODS
Nematode and bacterial strains
Wild O. tipulae strain JU1501 was isolated from a rotting apple from Kerarmel, Plouezoc’h, France (GPS coordinates 48.65151, −3.85573) on August 6, 2008. B. atropi type strain LUAb4 was isolated from JU1501 through cleaning of dauer animals to remove contaminating microbes in M9 buffer + 0.25% SDS, 50 ug/mL of carbenicillin, 25 ug/mL of kanamycin, 12.5 ug/mL of tetracyclin, 100ug/mL of gentamycin, 50 ug/mL of streptomycin, 37.5 ug/mL of chloramphenicol, and 200 ug/mL of cefotaxime33. After cleaning of JU1501, non-OP50-1 colonies were seen growing on nematode growth media (NGM) plates containing this strain. Single colonies were streaked to LB plates twice to ensure purity and the 16S rDNA was sequenced using primers 27F (AGAGTTTGATCMTGGCTCAG) and 1492R (GGTTACCTTGTTACGACTT).
Fluorescent in situ hybridization (FISH)
FISH was performed as described previously34. Probes to the small subunit rRNA of bacteria and microsporidia were conjugated to either CAL Fluor Red 610 (CF610) or 5-Carboxyfluorescein (FAM). The probes used were MicroA-CF610 (CTCTG TCCATCCTCGGCAA), MicroC-CF610 (CAGAATCAACCTGGTGCCTT), and MicroE-CF610 (GTACTGGAAATTCCGTGTTC), B. atropi-specific 16S probe b004 (TTATCCAGCGCCGTTTCTTTC), EUB338 (GCTGCCTCCCGTAGGAGT), and Alphaproteobacteria-specific 16S b002 (TGTACCGACCCTTAACGTTC).
Fitness assays
Lifespan assays were with conducted using a bleached strain of JU1501 to remove all horizontally transmitted microbes. Assays were conducted in technical triplicate across two separate trials with n=20 animals per plate seeded with either OP50-1 (the standard E. coli food source) or LUAb4 (B. atropi). Plates were grown at 23°C and animals were scored every 24 hours for death by touching non-motile animals with a pick. Accidentally killed and missing animals were censored from the count, but animals killed due to bagging were counted due to the possibility of infection-induced bagging. Brood size assays were conducted similarly, except n=20 animals per condition were plated to individual plates across two separate trials. The number of viable (hatched) progeny were counted every 24 hours and removed from the plate.
Standard pulse infection procedure
Two days prior to the infection, NGM plates were fully covered with 1 mL of an overnight culture of B. atropi strains or OP50-1 (OD600 ~ 0.4-0.5) and bacteria were allowed to grow into a full lawn at room temperature. On the day of infection, animals JU1501 grown on standard OP50-1 food source were collected with M9T buffer (M9 buffer, 0.05% TritonX-100), transferred onto B. atropi plates, and incubated 2 hrs at 23°C to allow infection to occur. Then, animals were washed off plates into 15 mL centrifuge tubes, washed 4 times with M9T for 20 minutes, and plated onto the OP50-1 plates. Animals are incubated at 23°C for indicated hours then processed by different assays and techniques as described below.
Pulse-chase infection time course
JU1501 animals were infected using the standard pulse infection procedure (see above). Animals were harvested at 16, 24, 36, and 48 hpi and FISH was performed as above with the B. atropi b004 probe. Images were taken and blinded for analysis, with animals binned as short filaments, long filaments, or filled with coccobacilli based on the majority phenotype seen in the animal. Uninfected animals or those with solely dispersed coccobacilli (representing recent invasion) were not counted. Samples were then unblinded and the percent of each phenotype at each timepoint was calculated separately for each replicate.
Transmission electron microscopy (TEM)
Animals were grown on OP50-1 to mixed stages were infected with wild-type B. atropi with the standard pulse infection procedure. At 24, 36, and 48 hours post infection, animals were harvested with M9 buffer, washed thoroughly with M9 for a couple times until the washing buffer looked sufficiently clear. Animals were then fixed with FGC fixative (2% paraformaldehyde, 2.5% glutaraldehyde in 0.1M cacodylate buffer pH 7.4) for 2 hours at room temperature on a rotator. Fixed samples were then kept in the same fixative at 4°C until further processing for TEM. TEM was performed by the Electron Microscopy Facility, Department of Cellular and Molecular Medicine at UCSD as described previously34.
Genome sequencing and assembly
B. atropi strain LUAb4 was cultured from a single colony in LB and DNA was purified using the DNeasy Blood and Tissue Kit (Qiagen). Libraries were made using Illumina Nextera DNA Library from ~700 bp fragments and sequenced on Illumina MiSeq 2×250 bp by GeneWiz Inc. Unprocessed reads were assembled with SPAdes (v3.13.0) using the ‘careful’ parameter and testing 21, 33, 55, 77, 99, and 127 kmers35. Annotation was conducted with prokka (v1.14.0) with the parameters ‘addgenes’ ‘genus Bordetella’, and an evalue of 1e-0636. This Whole Genome Shotgun project has been deposited at DDBJ/ENA/GenBank under the accession JAHPZX000000000. The version described in this paper is version JAHPZX010000000.
Phylogenomics analyses
Phylogenomics was conducted using the UBGC pipeline as described37, using 92 up-to-date bacterial core genes isolated from B. atropi and the following sequenced genomes: RHXM01000001.1 (A. aegrifaciens), UFQB01000001.1 (A. agilis), PYAL01000001.1 (A. aloeverae), AGUF01000105.1 (A. arsenitoxydans), CP013923.1 (A. denitrificans), VBUB01000010.1 (A. dolens), CP019325.1 (A. insolitus), GL982451.1 (A. insuavis), NJIG01000010.1 (A. marplatensis), QAYS01000001.1 (A. mucicolens), BCTK01000001.1 (A. piechaudii), CP017433.1 (A. ruhlandii), LGVG01000001.1 (A. spanius), LN831029.1 (A. xylosoxidans), CP013119.1 (Alcaligenes faecalis), FKIF01000001.1 (B. ansorpii), NC_010645.1 (B. avium), CP016170.1 (B. bronchialis), NC_019382.1 (B. bronchiseptica), CP016172.1 (B. flabilis), NEVR01000007.1 (B. genomosp. 1), NZ_CP012076.1 (B. hinzii), NZ_CP007494.1 (B. holmesii), NC_018828.1 (B. parapertussis), NC_002929.2 (B. pertussis), NC_010170.1 (B. petrii), NZ_CP016440.1 (B. pesudohinzii), and NZ_LT546645.1 (B. trematum). Alignments were made with RAxML based on amino acid sequences. Trees were made in MEGA X using maximum likelihood with 500 bootstraps using AA substitution via JTT model and tree inference using Nearest-Neighbor-Interchange.
Bacterial strains, plasmid construction, and gene knockout
B. atropi expressing tdTomato was created by mini-Tn7 tagging as describe before and the site of insertion was confirmed by arbitrary PCR and Sanger sequencing38.
In-frame deletion was carried out as described previously39. Briefly, 1.5-kb fragments upstream and downstream of genes of interest (including the first and last 5-10 codons, respectively) were cloned and performed Gibson assembly together with the triple-digested vector pCVD443 (NEBuilder HiFi DNA Assembly Cloning Kit E5520S, New England BioLabs Inc.). Assembly mixture was then used to transformed E. coli SM10 λpir by electroporation (MicroPulser Electroporator, Bio-Rad). The parental E. coli SM10 strain was used to mate with wild-type B. atropi. Exconjugants were selected for first recombination event with antibiotics and subsequently second recombination event with sucrose. Putative knockout colonies were confirmed for deletion of gene of interest by colony PCR with primers flanking the gene.
Complementation was performed by mating the filamentation mutant strain LUAb7 with E. coli SM10 that had been transformed with plasmid pANT4 constitutively expressing a wild-type copy of the gene gtaB.
In vitro filamentation assay
A single colony from a streaked plate was inoculated into an overnight culture for each bacterial strain. The overnight cultures (OD600 ~ 0.4-0.5) were diluted to OD600~ 0.2 with LB and 200 μL were used to seed 4.8 mL of either LB or TB media. Cultures were incubated at 32°C, 100 rpm. After 2 days, all cultures were blinded. Each blinded culture was resuspended gently by pipetting slowly with P1000 pipette once to avoid breaking filaments and 7 μL of the culture was mounted on glass slides for imaging with a fluorescent Nikon Ni-E Eclipse. For each condition, several random frames from the slide were taken and a total of 500 microbes or more were counted. These microbes could be either filaments (longer than 4 μm), elongated cells (less than 4 μm but longer than a typical coccobacillus), or coccobacilli (~0.5-1 μm). Only the filamentous microbes were counted toward the filament percentage, calculated using the ratio of the number of filamentous microbes to the total number of cells.
In vitro selection for filamentation mutants
Wild type B. atropi was subjected to filamentation induction by switching from LB to 5 mL of TB plus 200 μg/mL cefotaxime and grown at 32°C, 100 rpm for 2 days. Cultures were syringe filtered through a 5.0 μm PVDF membrane (Millex SV) with gentle, slow pressing and 200 ml of the flowthrough was used to seed 4.8 mL of TB plus cefotaxime for another cycle of induction. Between each selection cycle, cultures were analyzed post-filamentation induction by gently resuspending with P1000 pipette once and mounting 3 x 7 ml to determine the filament percentage as described above. If greater than 5% of the population filamented, then the culture went through another round of selection. If less than 5% filamented, the flowthrough was plated on LB to isolate single colonies. Select colonies were tested for in vitro filamentation in TB, leading to the isolation of LUAb4.
In vitro bacterial growth curve
Overnight cultures of either WT or LUAb7 were diluted to OD600 ~ 0.2 with LB. Each of the diluted cultures was added to 12 wells (total of 36) of a clear bottom, non-cell culture treated 96-well plate. The peripheral wells were added with sterile DI water to minimize evaporation during OD600 reading. OD600 values were taken at 1 hour interval for 36 hours at 32°C using tunable Versa max microplate reader (software SoftMax Pro 6.3) with settings for 30-second shaking before actual reading of the OD600. The final OD values at each time point for each condition was averaged from the 12 readings subtracted by the average blank reading (LB).
Intestinal cell-to-cell spreading assay
JU1501 was grown on OP50-1 food source and collected into a 15 mL centrifuge tube with M9T. Large animals (L3s, L4s, and adults) were allowed to settle to the bottom of the tube and the liquid on top containing mainly L1s and L2s was transferred to another 15 mL centrifuge tube. L1 and L2 animals were pelleted by centrifuging at 3000 x g for 1 minute and the animal pellets were divided into three parts and used for the standard pulse infection procedure as described above. After 2-hour pulse infection, animals were washed with MTEG buffer (M9T buffer, 0.25 mM EDTA, 10 μg/mL gentamycin) to kill extracellular bacteria. At 34 hpi, animals were collected for FISH.
FISH samples were scanned from the top right corner to the left, bidirectionally, to look for animals with distinguishable infection events. Each contiguous infection event is expected to result from a single cellular invasion, with a bacterium either filamenting or undergoing binary division resulting in a cluster of replicating coccobacilli. A total of 15 animals were imaged per condition, each containing between 1-10 distinguishable infection events. Images were taken with Zeiss LSM 710 inverted confocal microscope (software Zen 2012 SP1 Black edition, Zeiss LSM 710 release version 8.1.0.0) in z-stacks and analyzed with Fiji image software (version 2.1.0/1.53h) to count the number of whole intestinal nuclei that are fully passed by a single infection event along the A-P axis.
Normalized anterior-posterior (A-P) infection length
Animals were grown on OP50-1 food source and infected with standard pulse infection procedure (see above). At 34 hpi, animals fixed for FISH. Each condition was then imaged randomly for at least 30 animals with a fluorescent Nikon Ni-E Eclipse. Images were analyzed for normalized A-P infection length with Fiji image software (version 2.1.0/1.53h). In brief, for each animal in a particular condition, the distance between the most anterior and the most posterior points of a distinct, contiguous infection area was measured. If an animal had more than one contiguous infection area, the distances were averaged. This averaged A-P length of contiguous infection areas was then normalized to the length of the same infected animal to give the normalized A-P infection length.
Membrane dye and phalloidin staining of O. tipulae
Animal fixation and cuticle reduction were adapted from40. Worms were fixed with pre-chilled 4% paraformaldehyde in PBS at room temperature on a rotator for 30 minutes and moved to 4°C overnight. Animals were then washed 3 times with reduced cuticle buffer before incubating with fresh reduced cuticle buffer at 4°C for 24 hours. Afterwards, reduced animals were treated with 0.5 kU/mL collagenase type VII (C0773, Sigma Aldrich) at 37°C for ~32 hours. Afterwards, animals were rinsed once with DI water, followed by 3 washes with PBS, and store in PBS at 4°C for 1 day before staining. Animals were stained first with 0.5 mg/mL DAPI overnight. Excess DAPI was removed before staining with respective dyes. For membranes with a mixture of CellBrite Cytoplasmic membrane dye (Biotum) and BODIPY FL C5-Ceramide (Invitrogen) at 400- and 1000-fold dilution, respectively, for 2 days. For phalloidin staining, Alexa 488-tagged phalloidin (ThermoFisher, 400x stock) was added at 4x working concentration and incubated for 2 days. All the staining was carried out in a thermal shaker at 37°C, 900 rpm.
CFSE dye staining of O. tipulae
Animals were infected with the pulse-chase procedure as described above. After 2 hours of infection, animals were washed twice with MTEG buffer then wash once with M9T buffer. Animals were then pelleted down by spinning at 0.4x g for 30 seconds. 500 μL of CFSE staining buffer (M9, 2.5 mM serotonin, 40 μg/mL CFSE dye) was added and incubated for 3 hours. Animals were then plated on 6-cm NGM plate seeded with OP50 and another 500 !L of CFSE staining buffer was laid on top of the plate until animals were collected for FISH at 34 hpi.
Single nucleotide variation (SNV) calling
Strain LUAb7 was sequenced as described above using Illumina MiSeq. Reads were processed with cutadapt (v2.3) with parameters -u 10 -u -10 -U 10 -U 10 -m 50 to trim 10 bp from each end of every read and remove reads less than 50 bp41. Reads were mapped using bwa (v0.7.17-r1188) using the MarkDuplicates parameter42. SNVs were called using freebayes (v1.3.2-dirty) with parameter -C 50 requiring at least 50 supporting observations, a minimum mapping quality of 20, and base quality of 3043, with the resulting data annotated by hand to look for SNVs with >90% of reads containing the variation. Raw reads from LUAb7 sequencing are available at Sequence Reads Archive (SRA) accession SRR14751734.
DATA AVAILABILITY
This Whole Genome Shotgun project for B. atropi type strain LUAb4 has been deposited at DDBJ/ENA/GenBank under the accession XXXXXX. The version described in this paper is version XXXXXX. Raw reads from LUAb7 sequencing are available at Sequence Reads Archive (SRA) accession XXXXX. All data supporting this manuscript are available from the corresponding author upon request.
Funding
California State University, CSUPERB New Investigator Award and San Diego State University (SDSU) University Grants Program (UGP) award to RJL. MAF is an Investigator of the Centre National de la Recherche Scientifique, France. SDSU Rees-Stealy Research Fellowship (RSRF) and University Graduate Fellowship (UGF) award to TDT.
AUTHOR CONTRIBUTIONS
TDT, M-AF, RJL conceptualized the project. TDT, RJL designed the experiments. TDT, MAA, DL, RJL performed the experimental studies. TDT, RJL carried out data analysis and wrote of the manuscript.
COMPETING INTERESTS
Authors declare that they have no competing interests.
ACKNOWLEDGEMENT
We would like to thank Prof. Aharon Oren for his expertise in prokaryotic nomenclature and assistance in naming B. atropi. Thank you to Dalaena Rivera for helping come up with the name B. atropi. We would like to thank Dr. Anca Segall and Dr. Nick Shikuma for providing bacterial plasmids, access to equipment, and assistance with bacterial genetics. Thank you to Dr. Aaron Reinke for editing the manuscript.