Acizzia errabunda sp. nov. and Ctenarytaina insularis sp. nov.: Descriptions of two new species of psyllids (Hemiptera: Psylloidea) discovered on exotic host plants in New Zealand

Francesco Martoni; Karen F. Armstrong

doi:10.1371/journal.pone.0214220

Abstract

A recent molecular-based assessment of the psyllid fauna of New Zealand reported two genetically distinct, undescribed psyllid taxa on host plants not native to that country. Here, a morphological examination confirmed species-level variation that resulted in the description of two new psyllid species: Acizzia errabunda sp. nov. (Hemiptera: Psyllidae) from Acacia baileyana F. Muell and Ctenarytaina insularis sp. nov. (Hemiptera: Aphalaridae) from Syzygium smithii (Poir.) Nied. Furthermore, the examination of specimens from entomological collections and from observations recorded on an online database enabled a better understanding of the distribution and host plant associations of these psyllid species. The description of A. errabunda is based on material collected in both New Zealand and Australia from the same plant species, A. baileyana, whereas the psyllid C. insularis has been found to be present in Brunei and New Zealand on S. smithii and in New Caledonia on Melaleuca quinquenervia (Cav.) S. T. Blake.

Citation: Martoni F, Armstrong KF (2019) Acizzia errabunda sp. nov. and Ctenarytaina insularis sp. nov.: Descriptions of two new species of psyllids (Hemiptera: Psylloidea) discovered on exotic host plants in New Zealand. PLoS ONE 14(4): e0214220. https://doi.org/10.1371/journal.pone.0214220

Editor: Sean Michael Prager, University of Saskatchewan College of Agriculture and Bioresources, CANADA

Received: September 11, 2018; Accepted: March 8, 2019; Published: April 10, 2019

Copyright: © 2019 Martoni, Armstrong. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Data Availability: All the data required is present in the paper. Insects specimens are in the reported collection.

Funding: The authors received no specific funding for this work.

Competing interests: The authors have declared that no competing interests exist.

Introduction

The superfamily Psylloidea (Hemiptera: Sternorrhyncha) includes almost 4000 species described worldwide [1], with Australasia being a hotspot for the psyllid biodiversity [1, 2]. International interest in this group of hemipterans has increased since the discovery that some species are vectors of economically significant plant pathogens (e.g. [3–7]). This, coupled with climate change and globalization, has raised the risk of these species reaching areas and countries that would have not been inhabited a few decades ago [8–10]. As a consequence, psyllid taxonomy and systematics is of primary importance, not only for a better understanding of worldwide biodiversity, but also in order to recognise new or invasive species essential for international biosecurity and plant protection. Recent works on taxonomy and phylogenetics of psyllids have contributed towards this (e.g. [11–12]), including their placement within the order Hemiptera and their relationships with other hemipteroids [13].

Classification of the Psylloidea has been recently revised [11] and an increasing number of studies are using DNA sequence data to better understand the diversity and the phylogeny of taxa within it [12, 14–19]. Inevitably, new psyllid species are being described every year. For example, from the Hawaiian Islands 36 new species have been described in the genus Pariaconus [16] and seven in the genus Swezeyana [20], while 22 new species in the genera Acizzia, Myotrioza and Trioza have been described from Australia [14, 21].

The New Zealand psyllid fauna provides a good cross section of the worldwide psyllid biodiversity, including 24 genera across six of the eight families [22]. During the last 140 years, several taxonomists have described new species from this region (e.g. [23–26]). More recently, this group has come under close scrutiny in a biosecurity context due to the arrival there of the tomato/potato psyllid (TPP), Bactericera cockerelli Šulc. As vector of the plant pathogen ‘Candidatus Liberibacter solanacearum’, agent of the zebra chip disease, TPP has caused economically significant damage to New Zealand agriculture [7] and raised awareness of a need to know what species are present there [22].

A recent study of the New Zealand Psylloidea [18] used DNA barcoding [27] in support of morphological evidence and host plant associations to assess the biodiversity of this superfamily in the region. As a result, more than 20 new taxa were predicted to be new, undescribed species. Of these, two taxa were identified from host plants not native to New Zealand [18]. These were a Ctenarytaina sp. hosted by Syzygium smithii (Myrtaceae) a lilly pilly, but in New Zealand commonly known as ‘monkey apple’. Also an Acizzia sp. from Acacia baileyana (Fabaceae), the Cootamundra wattle. Both host plants are native to Australia [28], and therefore the origin of these psyllid species was initially considered to be from this country as well [18].

Worldwide, the genus Ctenarytaina (Aphalaridae) now includes 20 described species [1, 2] of which seven are present in New Zealand [22]. These are the endemic species Ctenarytaina fuchsiae (Maskell, 1890), C. pollicaris Ferris & Klyver 1932, and C. clavata Ferris & Klyver 1932, and the Australian native species C. eucalypti (Maskell, 1890), C. longicauda Taylor, 1987, C. spatulata Taylor, 1997 and C. thysanura Ferris & Klyver, 1932. Of all the Ctenarytaina psyllids worldwide, only one other species is associated with the plant genus Syzygium, being the recently described species C. fomenae from Western Cameroon [29]; there is no other Ctenarytaina associated with Melaleuca. Amongst other psyllid families, the species Trioza adventicia Tuthill, 1952 and Trioza eugeniae Froggatt, 1901 (both Triozidae) are the only other psyllids associated with Syzygium smithii [1, 22], while Trioza jambolanae Crawford, 1917 is associated with other Syzygium spp. in Bangladesh, China, India and West Himalaya [30, 31]. Similarly, the Australian psyllid Boreioglycaspis melaleucae (Moore, 1964) is the only other Aphalaridae sharing Melaleuca as the same host plant genus with C. insularis. In general, however, the association between psyllids of the genus Ctenarytaina and host plants of the family Myrtaceae is very well documented. For example, in Australia, many psyllid species in this genus are associated with Eucalyptus, such as C. spatulata Taylor, 1997, C. eucalypti, C. bipartita Burckhardt, Farnier, Queiroz, Taylor & Steinbauer, 2013, C. gracilis (Froggatt, 1901), C. longicauda, C. obscura (Froggatt, 1903) and C. peregrina Hodkinson, 2007 [2, 32].

The genus Acizzia (Psyllidae) includes 74 described species worldwide ([1]—excluding the Psylla taxa). The association between psyllids of the genus Acizzia and host plants of the family Fabaceae is strong, with at least 46 species documented as hosted by this legume family. Of these, 30 are on various plant species within the large Acacia genus [1]. Yen [33] suggested the number of Australian Acizzia spp. associated with Acacia may range between 58 and 77, however many of these species remain undescribed. New Zealand is home to 10 described species of Acizzia [22, 26]. These are Acizzia acaciae (Maskell, 1894), A. acaciaebaileyanae (Froggatt,1901), A. albizziae (Ferris & Klyver, 1932), A. conspicua Tuthill, 1952, A. dodonaeae Tuthill, 1952, A. exquisita Tuthill, 1952, A. hakeae Tuthill, 1952, A. jucunda Tuthill, 1952, A. solanicola Kent & Taylor, 1932 and A. uncatoides (Ferris & Klyver, 1932) [22, 34].

The species described here increase the number of taxa belonging to their respective genera in New Zealand. Therefore, the descriptions reported here are aimed to provide a tool for their identification while contributing to a better understanding of the New Zealand biodiversity.

Materials and methods

Materials collected

Psyllids collections were performed by beating plant leaves and branches on trays and by collecting the fallen insects using an entomological aspirator. After collection, all specimens were preserved in high grade ethanol and stored at -20°C.

One hundred six specimens of Ctenarytaina insularis sp. nov. were collected from two distinct locations in the urban area of Auckland and from one location in Wellington, New Zealand (Table 1). On the 21^st of February 2014 a first population was collected by S. Bulman (The New Zealand Institute of Plant and Food Research) from a Syzygium smithii in the urban area of Auckland, while a second population was collected by FM on the 23^rd of March 2015, in Fowlds Park, Auckland, also from S. smithii. A single psyllid was collected by FM on the 28^th of February 2016 on a Pittosporum eugenioides, in the urban area of Wellington, near Kelburn Park. A total of four specimens from these three locations, were previously used for DNA analysis [18] and partial sequences of the subunit 1 of the cytochrome oxidase gene (COI) are available on GenBank with accession numbers MG132452- MG132455. Additionally, samples from a fourth location (Auckland, New Zealand) previously collected by C.F. Hill (1997) on S. smithii and stored in high grade ethanol since that time, were provided by S. Bennett (New Zealand Ministry for Primary Industries, MPI) for examination (Table 1).

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Table 1. Species distribution and collection sites.

Country, location and host plant are reported for all the species examined in this study. This includes specimens collected by the authors (SC), loaned from museums and collections (SL) or provided by colleagues (SP), and observations reported on online database—only when including pictures that allowed identification (O). The star (*) highlights the only instance where a single insect was collected and, consequently, the host plant attribution is not confirmed.

https://doi.org/10.1371/journal.pone.0214220.t001

Eighty specimens of Acizzia errabunda sp. nov. were collected using the same procedure as above, from one location in South Australia (by FM and G. Taylor, 6^th of November 2014 near Mt Barker) and one in New Zealand (by FM, 17^th of July 2015 in the Mahoe Reserve, Lincoln, Canterbury), both from Acacia baileyana (Table 1). A total of six specimens, two from each of these populations, were previously used for DNA analysis [18] and partial sequences of COI are available on GenBank with accession numbers MG132221- MG132226. In addition to these, six individuals previously collected in Spring Grove, New Zealand, in December 2015 by H. Evans (following the same methods of [18]) were provided by C. Lange and S. Fowler (AgResearch Ltd) (Table 1). These specimens were preserved in high grade ethanol and had been stored at -20°C.

Materials examined from established collections

Additionally, samples belonging to different species were examined for a better understanding of the morphological differences between these and the newly described species. Multiple specimens of Acizzia acaciaebaileyanae (Froggatt, 1901), Acizzia jucunda (Tuthill, 1952), Ctenarytaina fuchsiae (Maskell, 1890), Ctenarytaina clavata Ferris & Klyver 1932 and Ctenarytaina pollicaris Ferris and Klyver 1932 from the Lincoln University Entomology Collection (LUNZ) were morphologically examined using the keys as detailed below. Furthermore, the holotype of Acizzia jucunda was provided by the New Zealand Arthropod Collection (NZAC), while the holotypes of Ctenarytaina distincta and C. lulla were obtained from the Bernice P. Bishop Museum of Honolulu, Hawaii (BPBM).

Unidentified specimens of Ctenarytaina spp. from New Zealand, New Caledonia and Brunei (details given below) were provided by the British Museum of Natural History (BMNH) in London, UK, together with specimens of Acizzia jucunda from Australia.

Preparation of specimens followed the work of Taylor and colleagues [14]. Morphology of adult characters followed Hodkinson and White [35] and that of immature characters followed White and Hodkinson [36]. Photographs were taken using a Nikon DS‐Ri2 camera connected to a Nikon SMZ25 microscope. Pictures were the result of stacking images using the software Nikon NIS‐Elements D v4.5. The magnification of each picture depended upon the dimension of the insects and of the morphological character of interest. Plates were prepared using GIMP version 2.8.14. Drawings were made using Inkscape v.0.92.3. All of the psyllid specimens collected, the holotypes and part of the paratypes have been deposited at the LUNZ. The remaining paratypes have been deposited at the BMNH.

Label data of holotypes are reported here using the conventions of Brown [37]: each label is delimited using quotes (‘…’), while lines are indicated with a solidus (/) and metadata are reported in curly brackets ({…}).

Nomenclatural acts

The electronic edition of this article conforms to the requirements of the amended International Code of Zoological Nomenclature (ICZN) [38, 39], and hence the new names contained herein are available under that Code from the electronic edition of this article. This published work and the nomenclatural acts it contains have been registered in ZooBank, the online registration system for the ICZN. The ZooBank LSIDs (Life Science Identifiers) can be resolved and the associated information viewed through any standard web browser by appending the LSID to the prefix “http://zoobank.org/”. The LSID for this publication is: urn:lsid:zoobank.org:pub:434FBA6F-A948-4005-824B-D5FD495BE6EC.

The electronic edition of this work was published in a journal with an ISSN and has been archived and is available from the following digital repositories: PubMed Central and LOCKSS.

Results

The specimens that were examined for this work, including museum specimens, and concluded to belong to the new species A. errabunda and C. insularis are reported in Table 1.

Taxonomy

Ctenarytaina insularis Martoni & Armstrong, 2019.

LSID: urn:lsid:zoobank.org:act:4419FC71-631B-42C9-84FF-FFDA7B91AEF7

(Figs 1, 2 and 3)

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Fig 1. Ctenarytaina insularis sp. nov.

Habitus dorsal view of female (A) and male (B); habitus lateral view of female (C) and male (D); wings of female (E) and male (F); head dorsal view of female (G) and male (H); lateral view of terminalia of female (I) and male (J). Scale bar length = 500μm (A-F) and 100μm (G-J).

https://doi.org/10.1371/journal.pone.0214220.g001

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Fig 2. Nymph of Ctenarytaina insularis sp. nov.

Habitus dorsal view (A) and habitus ventral view (B) with particular emphasis on the anal opening. Scale bar = 100μm.

https://doi.org/10.1371/journal.pone.0214220.g002

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Fig 3.

Details of terminalia for A. errabunda, female terminalia (A), anal ring (B) and male terminalia (C) with aedeaegus (D), and C. insularis, female terminalia (E), anal ring (F) and male terminalia (G) with aedeaegus (H) and inner side of paramere (I).

https://doi.org/10.1371/journal.pone.0214220.g003

Materials examined

Holotype: ♂ mounted on card triangle, deposited at the LUNZ. Labels: ‘NEW ZEALAND, AK / Auckland, Fowlds Park / 23 Mar 2015 F. Martoni / On Syzygium smithii.’ {Printed on white card}. ‘ID 127—Martoni F. 2017 / PhD Thesis. Lincoln University, / Canterbury–New Zealand.’ {Printed on white card}. ‘HOLOTYPE ♂ / Ctenarytaina insularis / Martoni & Armstrong 2019’ {Printed on red card}.

Paratypes: 3 ♀♀ mounted on card triangle, deposited at the LUNZ. Labels: ‘NEW ZEALAND, AK / Auckland, Fowlds Park / 23 Mar 2015 F. Martoni / On Syzygium smithii.’ {Printed on white card}, ‘ID 127—Martoni F. 2017 / PhD Thesis. Lincoln University, / Canterbury–New Zealand.’ {Printed on white card}, ‘PARATYPE ♀ / Ctenarytaina insularis / Martoni & Armstrong 2019’ {Printed on blue card}; 1 ♂, 1 ♀ mounted on microscope slide, deposited at the LUNZ. Labels: ‘PARATYPE / Ctenarytaina insularis / Martoni & Armstrong / 2019’ {Hand-written on white card}, ‘NEW ZEALAND, AK / Auckland—Mt Albert / 4 Nov 1997—C. F. Hill / on Syzygium smithii.’ {Hand-written on white card}; 2 ♂♂, 1 ♀ mounted on microscope slide, deposited at the LUNZ. Labels: ‘PARATYPE / Ctenarytaina insularis / Martoni & Armstrong / 2019’ {Hand-written on white card}, ‘NEW ZEALAND, AK / Auckland, Fowlds Park / 23 Mar 2015 F. Martoni / On Syzygium smithii.’ {Hand-written on white card}; 8 ♂♂, 5 ♀♀ mounted on 3 pins, deposited at the BMNH. Labels:

‘PARATYPE/ Ctenarytaina insularis / Martoni & Armstrong / 2019’ {Hand-written on white card}, ‘N. ZEALAND: / Auckland / Mt Albert / 26 VI 1997 / K. Froude leg P.Dale.’ [Hand-written on white card], ‘Acmena smithii.’ {Hand-written on white card}.

Diagnosis

Ctenarytaina insularis can be identified by the following combination of characters: small size, dark-brown colouration of the head and lighter (orange-yellowish) colouration to the rest of the body, rectangular vertex, and antennae as long as width of head. Female genitalia are shorter than the rest of abdomen, but of elongated shape and characterised by a pronounced post-anal bump and by both subgenital and proctiger tips pointing inward. The subgenital plate is shorter than the proctiger, which is straight and not downcurved. Male terminalia are pointy, with apical part of the parameres square and lacking setae on its inner border.

When compared with the Ctenarytaina species inhabiting New Zealand, the colour and size of C. insularis are similar to those of C. fuchsiae. The female terminalia of C. insularis (Figs 1I, 3E and 3F) are elongated in a similar way to those of C. fuchsiae (Fig 4B). However, they can be clearly distinguished by the more pronounced post-anal bump, by the tip of both subgenital plate and proctiger pointing inward (and not outward as in C. fuchsiae), and by the fact that the subgenital plate is shorter than the proctiger (Figs 1I, 3E and 3F). Similarly, the shape of the male terminalia of C. fuchsiae (Fig 4A) are differentiated by the tips of the parameres being pointy (and not rounded as in C. insularis, Figs 1J and 3G–3I), the shape of the proctiger being less rounded, and the lack of pronounced setae on its inner border. Additionally, the plant host for C. fuchsiae is Fuchsia excorticata (Onagraceae), while that for C. insularis is Syzygium smithii (Myrtaceae, see below). No New Zealand native Ctenarytaina are hosted by Syzygium. Rather, two species, C. pollicaris Ferris & Klyver, 1932 and C. clavata Ferris & Klyver, 1932, live on Kunzea spp. and Leptospermum spp. (both Myrtaceae) respectively. Compared to these other Ctenarytaina species, the dark orange/brown/yellow colour of C. insularis differs greatly from C. pollicaris, which is completely dark/black and C. clavata which is more uniformly yellow [26]. Also, while the female terminalia of C. insularis are slightly similar to those of C. pollicaris (Fig 4D), they narrow distinctively to a thin end immediately after the circum-anal ring. In addition, both the clavate male parameres of C. pollicaris (Fig 4C) and C. clavata (Fig 4E) differ greatly from the thin parameres of C. insularis.

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Fig 4.

Details of terminalia for C. fuchsiae, male terminalia (A), and female terminalia (B), C. pollicaris, male terminalia (C), and female terminalia (D), and C. clavata, male terminalia (E), and female terminalia (F). Scale bar length = 100μm.

https://doi.org/10.1371/journal.pone.0214220.g004

Outside New Zealand, the morphology of C. insularis appears closely related to those of C. lulla (Tuthill, 1942) and C. distincta (Tuthill, 1943), two species endemic to the Society Islands (French Polynesia). Despite these species being described solely based on female specimens [40, 41], the original description and the subsequent examination of the holotypes clearly identified these as different species. In fact, the female proctiger of C. distincta is down-curved (and not straight as in C. insularis; Figs 1I, 3E and 3F) and the subgenital plate is almost as long as the proctiger (while it is clearly shorter in C. insularis; Figs 1I, 3E and 3F). Additionally, upon inspection of the holotype, the colour of the body was darker, brown to dark brown, and the fore wing presented a darker band covering its proximal half (absent in C. insularis, Fig 1E and 1F). Similarly, C. lulla presents a vertex narrowed anteriorly (also shown in the original drawings [40]), antennae only ¾ of head’s width and female genitalia longer than the rest of abdomen; while C. insularis has rectangular vertex not narrowing anteriorly (Fig 1G and 1H), antennae as long as width of head (Fig 1G and 1H), and female genitalia shorter than rest of abdomen (Fig 1A, 1C and 1I). The holotype of C. lulla also showed a shorter vein M and longer veins M₁₊₂ and M₃₊₄, resulting in the cell m₁ being thinner and longer than that of C. insularis.

When considering the host plant association, the only other Syzygium-inhabiting Ctenarytaina is the recently described Ctenarytaina fomenae Soufo et al. 2018 [29], recorded in the African region of Western Cameroon. Beside the geographical separation between C. fomenae and C. insularis, the two species can be distinguished morphologically by the shape of the apical part of the parameres in C. insularis being straight and not slightly back turned as for C. fomenae.

A total of 83 specimens of C. insularis were identified amongst the samples provided by the BMNH. Of these, nine slide-mounted specimens (into three microscope slides) and 13 pinned specimens were originally collected in New Zealand in 1997 by K. Froude and P. Dale, from Syzygium smithii (Table 1). Another 32 slide-mounted specimens (into 20 microscope slides) and 14 pinned samples were collected from five different areas of New Caledonia in 1982 by D. Hollis, from Melaleuca quinquenervia (Myrtaceae) (Table 1). Lastly, five adult females and 10 nymphs (on four microscope slides) were collected from Syzygium in Brunei, on the 31^st of October 1992 by J.H. Martin, and provided by the BMNH. These, despite not including male specimens, could be unambiguously identified as C. insularis.

Colouration

Adult. Overall colour of the body dark orange/brown, with head and thorax dark brown or black while the abdomen remains of a lighter pale yellow (Fig 1A–1D). Eyes dark. Genal processes yellow. Antennae are light orange, with the last two segments dark brown. Wings are hyaline with darker veins (Fig 1E and 1F). Male terminalia are pale yellow. Female terminalia are darker, with an orange proctiger, similar to the colour of the thorax.

Nymphs. Habitus as in Fig 2. The cephalo-thoracic plate is light orange/yellow; eyes are red with a darker brownish spot laterally; antennae light orange/yellow, with the last two segments of a darker brown; thoracic sclerites just slightly darker than the rest of the body; forewing and hindwing pads almost white; caudal plate slightly glossy.

Structure

Adult. Body short and broad. Head: vertex short and broad, 0.45 times as long as wide; genal processes short and rounded. Antennae quite short, as long as head if not shorter. Thorax short and broad. Fore wing 2.35 times as long as width of head and 2.7 times as long as wide. Vein Rs longer than M (up to 1.6 times), both veins are straight and parallel with vein Cu1a, until Cu1a abruptly deviates to the margin of the wing. Male terminalia quite slender, with proctiger longer than parameres. Parameres thin and slender internally covered in setae, except for a triangular area at the base. Female terminalia straight and moderately long with proctiger longer than subgenital plate (up to 1.4 times), wider in the proximal part and narrow to the point.

Nymphs: Habitus as in Fig 2. Distribution of capitate setae on lateral margin of caudal plate shows 12 setae for each side divided into two groups of three setae and a caudal group of six. However, the six setae in caudal position for each side are grouped together with those of the other side, resulting in a group of 12 setae in caudal position (Fig 2). Circum-anal pore ring in ventral position (Fig 2B).

Measurements and ratios

Measurements are in mm (5 ♂, 5 ♀). Length of body (vertex to terminalia) ♂ 0.93–1.31, ♀ 1.01–1.44; length of body (vertex to apex of folded wings) ♂ 1.29–1.63, ♀ 1.55–1.92; width of head (HW) ♂ 0.55–0.58, ♀ 0.58–0.69; length of genal processes (GCL) ♂ 0.03–0.04, ♀ 0.04–0.05; length of vertex (VL) ♂ 0.14–0.16, ♀ 0.13–0.17; width of vertex (VW) ♂ 0.31–0.36, ♀ 0.35–0.37; length of antenna (AL) ♂ 0.53–0.57, ♀ 0.53–0.60; length of fore wing ♂ 1.25–1.33, ♀ 1.41–1.54; width of fore wing ♂ 0.45–0.51, ♀ 0.51–0.56; length of vein Rs ♂ 0.92–1.02, ♀ 1.08–1.18; length of vein M (M) ♂ 0.60–0.67, ♀ 0.67–0.76; length of vein M1+2 (M1) ♂ 0.24–0.31, ♀ 0.30–0.36; marginal width of cell m1 ♂ 0.12–0.17, ♀ 0.16–0.18; marginal width of cell cu1 ♂ 0.37–0.40, ♀ 0.41–0.49; length of vein Cu1b ♂ 0.09–0.14, ♀ 0.13–0.15; length (height) of proctiger (PL) ♂ 0.21–0.22; length of paramere ♂ 0.14–0.16; length of proximal aedeagal segment ♂ 0.29–0.31; length of distal aedeagal segment ♂ 0.06–0.09; length of proctiger (PL) ♀ 0.36–0.41; length of circum-anal ring (CL) ♀ 0.15–0.17; length of subgenital plate (SL) ♀ 0.29–0.34.

Ratios: GCL:VL ♂ 0.24–0.27, ♀ 0.24–0.31; VL:VW ♂ 0.40–0.49, ♀ 0.40–0.49; VL:HW ♂ 0.25–0.29, ♀ 0.22–0.30; AL:HW ♂ 0.97–1.01, ♀ 0.80–0.99; PL:HW ♂ 0.36–0.40, ♀ 0.53–0.70; PL:CL ♀ 2.40–2.52; PL:SL ♀ 1.08–1.40; WL:HW ♂ 2.31–2.41, ♀ 2.09–2.56; WL:WW ♂ 2.61–2.78, ♀ 2.68–2.84; Rs:M ♂ 1.45–1.61, ♀ 1.55–1.62; M1:M ♂ 0.37–0.49, ♀ 0.43–0.52.

Etymology

The latin word “insularis” means “of the island”. This was chosen since this psyllid was collected in Brunei, New Caledonia and in New Zealand, making it an “insular” psyllid.

Distribution

In New Zealand, Ctenarytaina insularis was collected for this study from four locations, all in the North Island (Table 1). Three of these were within the urban area of Auckland, including Mt. Albert and Fowlds Park, while the fourth was in Wellington. Additionally, populations from other areas of Auckland (Henderson Park and the suburb of St. John) were observed by S. Thorpe and pictures and information allowing identification were provided on the website iNaturalist (https://www.inaturalist.org). Other collections included 21 specimens from an urban area of Auckland (Mt. Albert), New Zealand, in 1997, by P. Dale and K. Froude on Syzygium smithii and 48 specimens from New Caledonia in 1982 by D. Hollis, on Melaleuca quinquenervia (Myrtaceae). Specifically, eight microscope slide-mounted samples were collected in the town of Hienghène, 26 samples (mounted on 12 slides) on Mt. Koghis, 12 pinned samples in the area of Noumea (Mt. Toro) and one sample each in Poum and near Tiebaghi mines (Table 1). All the specimens collected in Brunei were collected by J.H. Martin from the same location in the Temburong district, Sungai Temburong.

Host plant

All the specimens from New Zealand were collected from Syzygium smithii (Myrtaceae), except for a single specimen collected from Lemonwood (Pittosporum eugenioides), in Wellington. Considering that both immature stages and adult individuals were recorded in high numbers from S. smithii on multiple occasions, this plant is reported here as Ctenarytaina insularis’ host plant. This is in accordance with the definition of host plant made by Burckhardt and colleagues [42], stating that all the life stages must be present on the plant for it to be defined as host plant. Similarly, all the specimens from Brunei were collected from a Syzygium sp. and they included immature stages. On the other hand, the specimens from New Caledonia were collected from Melaleuca quinquenervia. These also included both immature stages and adults. While it is not extremely common for a psyllid species to have host plants belonging to different genera [43], it is not rare to record different host plants within the same family [43]. Therefore, considering that both M. quinquenervia and S. smithii belong to the family Myrtaceae, it is plausible to assume that these are both host plant to C. insularis in the respective countries.

Remarks

The first official report of Ctenarytaina insularis in New Zealand dates back to 2010 [34] as Ctenarytaina sp. on Syzygium. This was informed by field collections performed in the area of Auckland in 1997 (S. Bennett, personal communication), therefore this species is already included, as Ctenarytaina sp. within the 99 taxa reported in the most recent checklist of the New Zealand psyllids [22].

There are no reports for either Ctenarytaina spp. or Aphalaridae spp. in New Caledonia [1], therefore C. insularis would be the first member of this genus and family, there.