AMERICAN MUSEUM NOVITATES 


Number 3881, 26 pp. 


June 19, 2017 


A New Species of Nectar-feeding Bat of the Genus 
Hsunycteris (Phyllostomidae: Lonchophyllinae) from 

Northeastern Peru 

PAUL M. VELAZCO, 1 J. ANGEL SOTO-CENTENO, 1 DAVID W. FLECK, 2 
ROBERT S. VOSS, 1 AND NANCY B. SIMMONS 1 

ABSTRACT 

A new species of the nectarivorous bat genus Hsunycteris is described from lowland Ama¬ 
zonian forest in northeastern Peru. The new species, H. dashe, can be distinguished from other 
congeners by its larger size; V-shaped array of dermal chin papillae separated by a wide basal 
cleft; metacarpal V longer than metacarpal IV; broad rostrum; lateral margin of infraorbital 
foramen not projecting beyond rostral outline in dorsal view; well-developed sphenoidal crest; 
large outer upper incisors; weakly developed lingual cusp on P5; and well-developed, labially 
oriented Ml parastyle. A phylogenetic analysis of cytochrome -b sequence data indicates that 
H. dashe is sister to a clade that includes all other species of the genus including H. cadenai, H 
pattoni, and a paraphyletic H. thomasi. We provide a key based on craniodental and external 
characters of all four known species of Hsunycteris. 

INTRODUCTION 

The Neotropical bat genus Hsunycteris includes three described species of nectarivo¬ 
rous bats belonging to the phyllostomid subfamily Lonchophyllinae (Parlos et ah, 2014). 
The combined geographic ranges of these species extend from Panama to central Bolivia 
(Woodman and Timm, 2006). Hsunycteris species can be distinguished from other loncho- 
phyllines by a combination of the following characteristics: small size (GLS 19.5-22.5 mm, 

1 Division of Vertebrate Zoology (Mammalogy), American Museum of Natural History. 

2 Division of Anthropology, American Museum of Natural History. 

Copyright © American Museum of Natural History 2017 


ISSN 0003-0082 


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AMERICAN MUSEUM NOVITATES 


NO. 3881 


FA 30.0-34.0 mm), bases of dorsal pelage hairs paler than tips, uropatagium not conspicu¬ 
ously furred, rostrum shorter than braincase, infraorbital foramen above anterior root of 
the second upper premolar, first and second upper premolars elongated, and central cuspid 
of lower premolars not deflected labially (Parlos et ah, 2014; Cirranello et ah, 2016). Prior 
to the revision of Parlos et ah (2014), species of Hsunycteris were included in the genus 
Lonchophylla , but the latter taxon was found to be paraphyletic with respect to other lon- 
chophylline genera in numerous studies (Davalos and Jansa, 2004; Woodman and Timm, 
2006; Woodman, 2007; Davalos et ah, 2012; Davalos et ah, 2014). Parlos et ah (2014) 
described Hsunycteris to include three species of a previously unnamed clade that is the 
sister group of a larger clade comprising all other lonchophyllines ( Lonchophylla sensu 
stricto, Lionycteris, Xeronycteris, and Platalina ). 

As currently recognized, Hsunycteris comprises three species: H. cadenai, H. pattoni, and 
H. thomasi. Allen (1904) described Lonchophylla thomasi (= Hsunycteris thomasi ) based on one 
male specimen collected in the state of Bolivar, Venezuela. Hsunycteris thomasi is the most 
widespread species, with a distribution that almost matches that of the genus. Neither Wood¬ 
man and Timm (2006) nor Griffiths and Gardner (2008) recognized subspecies of H. thomasi, 
but several studies agree that it is most likely a paraphyletic species complex (Clare et ah, 2011; 
Parlos et ah, 2014). Parlos et ah (2014) analyzed mitochondrial and nuclear genes and identified 
two lineages in H. thomasi, one of which is apparently more closely related to H. pattoni than 
to the other putative lineage of H. thomasi. Since both lineages of H. thomasi include specimens 
collected close to the type locality for this species and no known morphological traits can be 
used to distinguished these lineages, it is difficult to determine which individuals correspond 
to H. thomasi sensu stricto and which represent an unnamed species. 

Woodman and Timm (2006) described the other two species of the genus. Hsunycteris 
cadenai is known from three localities in western Colombia (Woodman and Timm, 2006; 
Mantilla-Meluk et ah, 2010). Hsunycteris pattoni was originally described from a single speci¬ 
men from southeastern Peru, but is now known from five additional localities in Colombia, 
Ecuador, Peru, and Bolivia (Woodman and Timm, 2006; Mantilla-Meluk et ah, 2009; Mantilla- 
Meluk et ah, 2010; Parlos et ah, 2014). No subspecies are recognized in either species (Parlos 
et ah, 2014). 

Recent faunal inventory work in the Yavari-Ucayali interfluvial region of the Peruvian 
Amazon has resulted in the collection of three specimens of Hsunycteris that do not fit the 
diagnosis of any previously described species in the genus. We analyzed morphological, mor¬ 
phometric, and molecular data to describe these specimens as representing a new species of 
Hsunycteris and place this new taxon in phylogenetic context. 


MATERIAL AND METHODS 

Our study employed analyses of mitochondrial gene sequences as well as standard mor¬ 
phological comparisons. The specimens examined and tissues used for this study belong to the 
following collections: 


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VELAZCO ET AL.: NEW SPECIES OF HSUNYCTERIS 


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AMNH, AMCC 
ASNHC, ASK 

CEBIOMAS 

CM 

FMNH 

KU 

LSUMZ, M 

MUSA 

MUSM 

MVZ 

QCAZ 

ROM 
TTU, TK 
UMMZ 
USNM 


American Museum of Natural History, New York, New York 

Angelo State Natural History Collections, Angelo State University, San 

Angelo, Texas 

Centro de Ecologia y Biodiversidad, Lima, Peru 

Carnegie Museum of Natural History, Pittsburgh, Pennsylvania 

Field Museum of Natural History, Chicago, Illinois 

Biodiversity Institute & Natural History Museum, University of Kansas, 
Lawrence, Kansas 

Museum of Natural Science, Louisiana State University, Baton Rouge, 
Louisiana 

Museo de Historia Natural, Universidad Nacional de San Agustin, Arequipa, 
Peru 

Museo de Historia Natural de la Universidad Nacional Mayor de San Mar¬ 
cos, Lima, Peru 

Museum of Vertebrate Zoology, University of California, Berkeley, 
California 

Museo de Zoologia of the Pontificia Universidad Catolica del Ecuador, 
Quito, Ecuador 

Royal Ontario Museum, Toronto, Ontario, Canada 

Museum of Texas Tech University, Lubbock, Texas 

Museum of Zoology, University of Michigan, Ann Arbor, Michigan 

National Museum of Natural History, Smithsonian Institution, Washington, 

D.C. 


Morphological Analyses 

We examined 102 specimens of adult Hsunycteris (56 males and 46 females; appendix 1) 
and evaluated external and osteological characters including, but not restricted to, those defined 
by Wetterer et al. (2000), Woodman and Timm (2006), and Davalos et al. (2014). Dental 
homology nomenclature for the premolars in the discussions below follows that of Davalos et 
al. (2014): 1st upper premolar (P4), 2nd upper premolar (P5), 1st lower premolar (pi), 2nd 
lower premolar (p4), and 3rd lower premolar (p5). All measurements reported herein are from 
adult individuals with closed epiphyses unless otherwise indicated. The first four measurements 
listed below were taken from skin labels or other records made by the original collector; all 
other measurements were taken by us using digital calipers and were recorded to the nearest 
0.01 mm. Linear measurements are given in millimeters (mm), and weights are reported in 
grams (g). Descriptive statistics (mean and observed range) were calculated for all samples. 
Measurements are defined as follows: 


Total length (TL): Distance from the tip of the snout to the tip of the last caudal vertebra. 


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AMERICAN MUSEUM NOVITATES 


NO. 3881 


Length of tail (LT): Measured from the point of dorsal flexure of the tail with the sacrum to the 
tip of the last caudal vertebra. 

Hind-foot length (HF): Measured from the anterior edge of the base of the calcar to the tip of 
the claw of the longest toe. 

Ear length (Ear): Measured from the ear notch to the fleshy tip of the pinna. 

Forearm length (FA): Distance from the elbow (tip of the olecranon process) to the wrist 
(including the carpals). This measurement is made with the wing at least partially folded. 
Greatest length of skull (GLS): Distance from the posteriormost point on the occiput to the 
anteriormost point on the premaxilla (excluding the incisors). 

Condyloincisive length (CIL): Distance between a line connecting the posteriormost margins of 
the occipital condyles and the anteriormost point on the upper incisors. 

Condylocanine length (CCL): Distance between a line connecting the posteriormost margins of 
the occipital condyles and a line connecting the anteriormost surface of the upper canines. 
Braincase Breadth (BB): Greatest breadth of the globular part of the braincase, excluding mas¬ 
toid and paraoccipital processes. 

Width at Canines (C-C): Greatest breadth across the outer margins of the alveoli of upper 
canines. 

Mastoid Process Width (MPW): Greatest breadth across the mastoid processes. 

Maxillary Toothrow Length (MTRL): Distance from the anteriormost surface of the upper 
canine to the posteriormost surface of the crown of M3. 

Width at M2 (M2-M2): Greatest width of palate across labial margins of the M2s. 

Dentary Length (DENL): Distance from midpoint of condyle to the anteriormost point of the 
dentary. 

Mandibular Toothrow Length (MANDL): Distance from the anteriormost surface of the lower 
canine to the posteriormost surface of m3. 

Coronoid Height (COH): Perpendicular height from the ventral margin of mandible to the tip 
of the coronoid process. 

All measurements were log-transformed to achieve normalization for statistical analyses. 
We evaluated differences between sexes and among species by principal component analysis 
(PCA) using a correlation matrix. Components with eigenvalues greater than 1 were retained. 
Principal component (PC) scores were plotted to show relationships between species groups 
in morphospace. Analyses were performed using PAST v3.01 (Hammer et al., 2001). We con¬ 
structed a dichotomous identification key for all of the named species of Hsunycteris based on 
morphological traits identified during the course of the study. 


Molecular Analyses 

Field-collected frozen muscle and liver tissues preserved in EtOH of specimens cataloged 
as Lonchophylla mordax, L. pattoni, and L. thomasi were obtained for genetic analysis. DNA 
was extracted from small pieces of tissue (-5-10 mg) for each specimen using standard pro- 


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TABLE 1. Species, tissue/collection number, locality information, and GenBank accession numbers for the 
Hsunycteris and outgroup samples used in the molecular portion of this study. 


Taxon 

Tissue/Collection Numbers 3 

Locality 13 

GenBank 

Glossophaga soricina 

TK 104054/TTU 84826 

Ecuador: Pastaza (22) 

KF815298 d 

Lionycteris spurrelli 

TK 22540/TTU 39123 

Panama: Darien (29) 

KF815283 d 

Lionycteris spurrelli 

TK 22550/TTU 39129 

Panama: Darien (29) 

KF815284 d 

Lionycteris spurrelli 

TK 22549/TTU 39128 

Panama: Darien (29) 

KF815304 d 

Platalina genovensium 

TK 161667/MUSA 9383 

Peru: Arequipa (32) 

KF815311 d 

Xeronycteris vieirai 

MVZ 186020 

Brazil: Paraiba (10) 

KF815312 d 

Lonchophylla chocoana 

ROM 105786 

Ecuador: Esmeraldas (13) 

AF423092 c 

Lonchophylla concava 

TK 104601/QCAZ 9087 

Ecuador: Esmeraldas (16) 

KF815280 d 

Lonchophylla concava 

TK 104602/QCAZ 9568 

Ecuador: Esmeraldas (16) 

KF815281 d 

Lonchophylla concava 

TK 104612/QCAZ 9088 

Ecuador: Esmeraldas (17) 

KF815305 d 

Lonchophylla concava 

TK 135677/TTU102960 

Ecuador: Esmeraldas (14) 

KF815282 d 

Lonchophylla handleyi 

TK 22611/TTU 46169 

Peru: Huanuco (33) 

KF815285 d 

Lonchophylla hesperia 

M921/LSUMZ 27253 

Peru: Lambayeque (34) 

KF815310 d 

Lonchophylla orienticollina 

ASK 7733/QCAZ 8566 

Ecuador: Morona Santiago (19) 

KF815291 d 

Lonchophylla orienticollina 

ASK 7737/QCAZ 8570 

Ecuador: Morona Santiago (19) 

KF815308 d 

Lonchophylla robusta 

QCAZ 5406 

Ecuador: Pichincha (24) 

KF815313 d 

Lonchophylla robusta 

TK 104594/TTU 85366 

Ecuador: Esmeraldas (16) 

KF815286 d 

Lonchophylla robusta 

TK 104600/QCAZ 9085 

Ecuador: Esmeraldas (16) 

KF815287 d 

Lonchophylla robusta 

TK 104619/TTU 85391 

Ecuador: Esmeraldas (17) 

KF815306 d 

Lonchophylla robusta 

TK 135515/QCAZ 9091 

Ecuador: Esmeraldas (14) 

KF815288 d 

Lonchophylla robusta 

TK 135516/QCAZ 9092 

Ecuador: Esmeraldas (14) 

KF815289 d 

Lonchophylla robusta 

TK 135658/TTU 102941 

Ecuador: Esmeraldas (14) 

KF815290 d 

Hsunycteris cadenai 

TK 135800/QCAZ 9097 

Ecuador: Esmeraldas (15) 

KF815297 d 

Hsunycteris cadenai 

TK 104675/QCAZ 9096 

Ecuador: Esmeraldas (18) 

KF815307 d 

Hsunycteris cadenai 

TK 104676/TTU 85448 

Ecuador: Esmeraldas (18) 

KF815295 d 

Hsunycteris cadenai 

TK 104679/TTU 85451 

Ecuador: Esmeraldas (18) 

KF815296 d 

Hsunycteris dashe 

AMCC 109488/MUSM 15206 

Peru: Loreto (35) 

MF062529 e 

Hsunycteris dashe 

AMCC 109608/AMNH 273165 

Peru: Loreto (35) 

MF062528 e 

Hsunycteris pattoni 

AMNH 209358 

Bolivia: Beni (1) 

AF423084 c 

Hsunycteris pattoni 

AMNH 278465 

Peru: Loreto (39) 

MF062534 e 

Hsunycteris pattoni 

AMNH 278500 

Peru: Loreto (39) 

MF062533 e 

Hsunycteris pattoni 

AMCC 109525/AMNH 273069 

Peru: Loreto (35) 

MF062532 e 

Hsunycteris pattoni 

AMCC 109557/AMNH 273093 

Peru: Loreto (35) 

MF062531 e 

Hsunycteris pattoni 

CEBIOMAS 100 

Peru: Loreto (39) 

MF062536 e 

Hsunycteris pattoni 

CEBIOMAS 101 

Peru: Loreto (39) 

MF062537 e 

Hsunycteris pattoni 

KU 144232/MUSM 24350 

Peru: Madre de Dios (42) 

KF815314 d 

Hsunycteris pattoni 

AMCC 109713/MUSM 13205 

Peru: Loreto (35) 

MF062530 e 


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AMERICAN MUSEUM NOVITATES 


NO. 3881 


Taxon 

Tissue/Collection Numbers 3 

Locality 13 

GenBank 

Hsunycteris pattoni 

AMCC 109527/MUSM 15207 

Peru: Loreto (35) 

MF062535 e 

Hsunycteris pattoni 

MVZ 192651/UMMZ 160710 

Peru: Madre de Dios (41) 

KF815309 d 

Hsunycteris thomasi 

KU 158056 

Peru: Loreto (40) 

KF815292 d 

Hsunycteris thomasi 

KU 158058 

Peru: Loreto (40) 

KF815315 d 

Hsunycteris thomasi 

TK104012/TTU 84784 

Ecuador: Pastaza (21) 

KF815293 d 

Hsunycteris thomasi 

AMCC 110340/AMNH 267940 

French Guiana: Cayenne (25) 

MF062539 e 

Hsunycteris thomasi 

AMCC 110262/AMNH 267943 

French Guiana: Cayenne (25) 

AF423086 c 

Hsunycteris thomasi 

KU 155154 

Guyana: Potaro-Siparuni (27) 

KF815294 d 

Hsunycteris thomasi 

TK 10310/CM 63723 

Surinam: Nickerie (45) 

KF815299 d 

Hsunycteris thomasi 

TK 10425/CM 63713 

Surinam: Brokopondo (43) 

KF815300 d 

Hsunycteris thomasi 

TK 17530/CM 76778 

Surinam: Brokopondo (44) 

KF815301 d 

Hsunycteris thomasi 

TK 17539/CM 76779 

Surinam: Brokopondo (44) 

KF815302 d 

Hsunycteris thomasi 

TK 19267/CM 78396 

Venezuela: Bolivar (56) 

KF815303 d 


a Alphanumeric identifiers used by institutional tissue collections (and to label terminal in accompanying tree; fig. 6). 
See Material and Methods for names of museum collections identified by abbreviations in this table. 
b Country and next-largest administrative unit (stated, department, province, etc.). Numbers in parentheses refer to gaz¬ 
etteer entries (appendix 2), which provide additional geographic information. 
c Davalos and Jansa (2004). 
d Parlos et al. (2014). 
e This study. 


tocols of the QIAmp DNA Micro Kit (QIAGEN, Valencia, CA). Genomic DNA extractions 
were used as a template in polymerase chain reactions (PCR) to amplify the mitochondrial 
gene cytochrome b ( Cyt-b , 1140 bp). Primers used in PCR amplification of Cyt-b were MVZ05 
and UMMZ04 (Jansa et al., 1999). We integrated a series of overlapping 200 bp fragments 
(primers BATL4, BATH4, BATL5, and BATH5) from Davalos and Jansa (2004) to improve the 
confidence of the sequence reads. 

Polymerase chain reactions (PCR) were performed in a total volume of 25pi using DreamTaq 
polymerase mix (Thermo-Fisher Scientific, Waltham, MA), lpl of each primer at 0.1 pM, and lpl 
of template DNA. Thermal cycler conditions to amplify Cyt-b consisted of an initial denaturation 
of 95°C for 10 min, followed by 35 cycles of denaturation at 95° C for 20 s, annealing at 48° C for 
40 s, and elongation at 72° C for 1 min, and a final elongation step at 72° C for 10 min. PCR 
products were purified using ExoSAP-IT (USB Corporation, Cleveland, OH). Standard sequenc¬ 
ing reactions were carried out at the Sackler Institute of Comparative Genomics (section 19) at 
American Museum of Natural History following ABI Prism BigDye Terminator cycle sequencing 
protocols (Applied Biosystems, Foster City, CA). All sequences were annotated, aligned, and 
contigs assembled in Geneious R8 v8.1.8 (www.geneious.com; Kearse et al., 2012). 

Phylogenetic analyses were performed by combining the full Cyt-b sequences produced 
in this study with full and partial sequences available in GenBank from Davalos and Jansa 
(2004) and Parlos et al. (2014; table 1). We determined the best-fit model of nucleotide sub¬ 
stitution using the Akaike Information Criterion (AIC) in jModelTest v2.1 (Posada, 2008). 


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Model selection resulted in HKY+I+G, which we implemented in Bayesian and Maximum 
Likelihood (ML) phylogenetic analyses rooted using a sequence of Glossophaga soricina (TK 
104054) as outgroup. 

Bayesian phylogeny estimation was performed using MrBayes v3.2 (Ronquist et al., 2012) 
consisting of two independent runs of Metropolis-coupled Markov-chain Monte Carlo (MCMC) 
with four Markov chains. Each run was set for 10 million generations and sampling trees every 
1000 generations. The average standard deviation of split frequencies was 0.008, indicating con¬ 
vergence of the analysis. Further assessment of stationarity was performed in Tracer vl.6 (Ram- 
baut and Drummond, 2007) by examining log likelihood (In L) scores. The first 20% of the 
estimated topologies were discarded as burn-in and a consensus Bayesian tree was constructed. 

Maximum-likelihood (ML) analysis was performed using Garli v2.1(Bazinet et al., 2014). 
Parameter settings included a heuristic search of four replicates over 5 x 10 6 generations and 
a ML starting tree inferred from stepwise addition sequence. Other parameters were set as 
default. Nodal support for ML estimation was evaluated using 100 replicates of nonparametric 
bootstrap analysis. A majority-rule consensus tree of bootstrap replicates was constructed in 
the R package “ape” (analyses of phylogenetics and evolution) ver. 4.1 (Paradis, 2012). 

Finally, we estimated average uncorrected (p) and K2P pairwise distances using the R 
package ape v4.1 (Paradis, 2012). We trimmed all sequences in this analysis to the length of 
the shortest sequence (400 bp). These estimates were used to compare genetic distances of 
specimens collected within the Yavari-Ucayali interfluvial region, and between these and other 
previously defined Hsunycteris groups in Parlos et al. (2014). 

SYSTEMATICS 

Family Phyllostomidae Gray, 1825 

Subfamily Lonchophyllinae Griffiths, 1982 

Tribe Hsunycterini Parlos et al., 2014 

Genus Hsunycteris Parlos et al., 2014 

Hsunycteris dashe, new species 

Dashes nectar-feeding bat 

Lonchophylla mordax: Fleck et al., 2002: 96. 

Hsunycteris sp. nov.: Voss et al, 2016: 11. 

Holotype: The holotype (MUSM 15206; figs. 1, 3A, 4A), an adult female specimen pre¬ 
served in alcohol with the skull removed and cleaned, was collected by David W. Fleck (original 
number: DWF 380) on 2 September 1999 at Nuevo San Juan (73°9'50"W, 5°14'50"S; 150 m 
above sea level), a Matses village on the right (SE) bank of the Rio Galvez in the Peruvian 
department of Loreto (fig. 2). Frozen tissues are deposited at the Ambrose Monell Cryo Col¬ 
lection of the American Museum of Natural History (AMCC 109488). 


AMERICAN MUSEUM NOVITATES 


NO. 3881 


FIGURE 1. Dorsal and ventral views of the cranium and lateral view of the cranium and mandible of Hsun- 
ycteris dashe (MUSM 15206, holotype). Scale bar = 5 mm. 


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FIGURE 2. Map showing collecting localities of Hsunycteris species within the Yavari-Ucayali interfluvial 
region (boundaries highlighted in gray). See appendix 2 for locality names and geographic coordinates. The 
arrow indicates the type locality of H. dashe. 

Paratypes: Two additional specimens, a lactating adult female (AMNH 273165 [DWF 
662]) and her female pup (MUSM 15211 [DWF 663]), were collected at the type locality by 
David W. Fleck on 21 October 1999. The adult paratype (AMNH 273165), preserved in alcohol 
with the skull removed and cleaned, is accompanied by frozen tissues deposited at the Ambrose 
Monell Cryo Collection of the American Museum of Natural History (AMCC 109608). The 
juvenile paratype (MUSM 15211) is preserved in alcohol. 


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AMERICAN MUSEUM NOVITATES 


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A 


B 


FIGURE 3. Anterior views of the chins of Hsunycteris dashe (A, AMNH 273165) and H. pattoni (B, MUSM 
13205) illustrating taxonomic differences in the arrangement of the dermal papillae. In H. dashe the chin has 
several small dermal papillae arranged in a V and separated by a wide basal cleft. In H. pattoni, however the 
dermal papillae on the chin are larger and are not separated by a basal cleft. 

Distribution: Hsunycteris dashe is known only from the vicinity of the type locality in 
the Yavari-Ucayali interfluvial region of the Peruvian Amazon (fig. 2). 

Diagnosis and Description: Hsunycteris dashe is the largest species in the genus (FA 35-36 
mm; tables 2-3). Dorsal pelage 9-10 mm long, fur distinctly bicolored with pale pinkish bases 
(20% of length) and pale brown tips; ventral pelage 7 mm long, similar in color to the dorsal 
pelage, bicolored with pale pinkish bases (30% of length) and pale brown tips. Two interramal 
vibrissae present; genal vibrissae absent. Central rib of noseleaf weakly defined from lateral por¬ 
tions, extending from apex to edge of upper lip. Chin with several small dermal papillae arranged 
in a V shape and separated by a wide cleft (fig. 3A). Antero-internal surface of pinna sparsely 
covered with long hairs. Dorsal surface of the forearm naked. Metacarpal formula III > V > IV. 
Dorsal surface of uropatagium naked. Dorsal surface of foot sparsely covered by short hairs. 

Skull with broad rostrum; postorbital region not inflated and lacking lateral projections 
(fig. 1). Lateral margin of infraorbital foramen not projecting beyond rostral outline in dorsal 
view. Sphenoidal crest (Giannini et al., 2006: fig. 10) well developed. Posterior border of hard 
palate V-shaped. Left and right basisphenoid pits separated by narrow septum. Dentary deep, 
coronoid process low (slightly above level of articular condyle), and angular process broad. 

Dental formula 12/2, Cl/1, P2/3, M3/3 x 2 = 34 or 12/2, Cl/1, P3/3, M3/3 x 2 = 36. 3 
Inner and outer upper incisors not in contact. Outer upper incisors relatively large. P4 lin¬ 
gual cusp absent; P5 lingual cusp weakly developed; small gap present between P5 and Ml 
(fig. 4A). Ml parastyle well developed and labially oriented; Ml and M2 with broad proto¬ 
cone basin; M3 large; palate posterior to M3 shorter than the length of M3 (figs. 1, 4A). 

3 The former dental formula characterizes the adult paratype, and it is the usual formula in other congeneric 
species, whereas the holotype has an additional pair of small upper premolars (figs. 1, 4A). With only two 
adult specimens in hand, it is obviously impossible to determine which formula predominates in the species, 
although we suspect that the small anterior premolars of the holotype are supernumerary teeth, which com¬ 
monly occur in other lonchophyllines (Phillips, 1971; Nogueira et al., 2014). 


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TABLE 2. Measurements (mm) and weights (g) of the type series of Hsunycteris dashe. 


MUSM 

15206 9 a 

AMNH 

273165$ b 

MUSM 

15211 9 b > c 

TL 

61.0 

65.0 

45.0 

LT 

12.0 

8.0 

5.0 

HF 

11.0 

10.0 

9.0 

Ear 

13.0 

14.0 

10.0 

FA 

35.0 

36.0 

23.0 

GLS 

20.8 

20.5 

- 

CIL 

19.8 

19.8 

- 

CCL 

18.9 

18.9 

- 

BB 

8.7 

8.5 

- 

C-C 

4.0 

4.0 

- 

MPW 

8.9 

8.9 

- 

MTRL 

6.4 

6.5 

- 

M2-M2 

5.5 

5.5 

- 

DENL 

13.6 

13.7 

- 

MANDL 

6.8 

6.8 

- 

COH 

3.6 

3.8 

- 

Weight 

9.3 

10.2 

3.7 


a Holotype. 
b Paratype. 

c Juvenile, pup of AMNH 273165. 

Lower incisors large and broad. Distal cusp weakly developed on pi. Anterior cusp of p4 
oriented horizontally. Protoconid labially oriented on ml; ml paracristid notch strongly 
developed. Hypoconid wide on m2. 

Comparisons: External and craniodental measurements for Hsunycteris dashe and other 
congeneric species are provided in tables 2 and 3. Hsunycteris dashe can be easily distinguished 
from all other species of Hsunycteris by its longer forearm. However, there is substantial overlap 
among all Hsunycteris species in craniodental measurements, with H. dashe falling at the larger 
end of the spectrum for most variables. 

Externally, Hsunycteris dashe is distinguished from all other species in the genus by having 
longer hairs between the shoulders (9-10 mm, versus 7-8 mm in H. cadenai, H. pattoni, and H. 
thomasi ). The central rib of the noseleaf extends from the tip of the spear to the edge of the upper 
lip in H. dashe and H. thomasi, and it is weakly defined from the lateral portions of the noseleaf. 
In contrast, the central rib of the noseleaf is well defined but does not reach the edge of the upper 
lip in H. pattoni, and a distinct central rib is absent in H. cadenai. The chin has several small 
dermal papillae arranged in a V and separated by a wide basal cleft in H. dashe (fig. 3A), whereas 
the dermal papillae are larger and not separated by a basal cleft in H. cadenai, H. pattoni, and H. 
thomasi (fig. 3B). The antero-internal surface of each pinna is sparsely covered with long hairs in 
H. dashe, H. cadenai, and H. thomasi, whereas these hairs are more abundant in H. pattoni. Lastly, 


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TABLE 3. Measurements (mm) and weights (g) of three species of Hsunycteris. 


H. cadenai 

H. pattoni 

H. thomasi 


Females 3 

Males b 

Females c 

Males d 

Females e 

Males f 

TL 

62 (59-65) 2 

61, 60 

60 (50-67) 17 

59 (50-68) 19 

58 (49-65) 18 

59 (53-64) 29 

LT 

8 (7-9) 2 

10, 8 

8(5-10) 16 

7(5-9)19 

6 (4-9) 18 

7(4-11) 29 

HF 

8(8)5 

10, 8 

9(7-11)17 

9(8-10)19 

9 (7-11) 17 

9(7-11)30 

Ear 

14 (14) 2 

14, 15 

15 (12-17)17 

14 (12-16)19 

15 (11-16) 18 

15 (12-18)28 

FA 

32.1 (31.6- 
32.7) 5 

31.0,31.0 

32.8 (31.0-34.0) 
17 

32.0 (31.0- 
34.0) 19 

32.3 (30.6-34.3) 
18 

31.7 (29.7-33.5) 
32 

GLS 

21.1 (20.7- 
21.7) 3 

21.2,21.3 

20.8 (19.9-21.8) 
14 

20.6 (19.7- 
21.1) 9 

20.7 (19.6-21.7) 
17 

20.8 (19.7-21.9) 

33 

CIL 

20.6 (20.2- 
20.9) 2 

20.1, 20.6 

20.2 (19.2-21.2) 
12 

20.0 (19.4- 
20.4) 9 

19.9 (18.8-20.8) 
16 

20.1 (19.1-21.1) 

31 

CCL 

19.5 (19.1- 
19.8) 2 

19.0, 19.5 

19.2 (18.4-20.2) 
12 

19.1 (18.5- 
19.8) 9 

18.9 (17.9-19.7) 
17 

19.1 (18.1-20.1) 

33 

BB 

8.6 (8.4-9.0) 3 

8.8, 8.7 

8.2 (7.9-8.5) 14 

8.4 (8.2-8.6) 9 

8.2 (7.7-8.7) 18 

8.3 (8.0-8.6) 33 

C-C 

3.8 (3.7-3.9) 4 

3.9, 4.0 

3.7 (3.5-3.9) 11 

3.7 (3.6-3.8) 9 

3.7 (3.4-4.1) 17 

3.8 (3.5-4.2) 31 

MPW 

9.1 (9.1) 3 

9.1, 9.3 

8.7 (8.2-9.4) 14 

8.8 (8.5-8.9) 9 

8.5 (8.0-8.8) 17 

8.7 (8.3-9.0) 33 

MTRL 

6.8 (6.7-6.9) 3 

6.9, 7.0 

6.9 (6.5-7.3) 12 

6.7 (6.5-7.2) 9 

6.6 (6.3-7.1) 18 

6.7 (6.1-7.2) 33 

M2-M2 

5.1 (5.0-5.3) 3 

5.4, 5.3 

5.3 (5.0-5.7) 14 

5.2 (4.9-5.5) 9 

5.1 (4.8-5.3) 16 

5.2 (4.9-5.7) 32 

DENL 

14.4 (14.1- 
14.5) 3 

14.0, 14.5 

14.2 (13.5-15.0) 
13 

14.1 (13.8- 
14.6) 9 

13.9(13.0-14.7) 

15 

14.2 (13.4-14.9) 
32 

MANDL 

7.2 (7.1-7.3) 3 

7.2, 7.5 

7.2 (6.9-7.5) 13 

7.1 (6.8-7.9) 9 

6.9 (6.6-7.3) 16 

7.1 (6.8-7.6) 32 

COH 

3.9 (3.7-4.0) 3 

4.0, 4.0 

3.5 (3.0-3.9) 14 

3.6 (3.3-3.9) 9 

3.5 (3.1-4.0) 16 

3.7 (3.3-4.0) 32 

Weight 

— 


7.9 (5.0-15.0) 

16 

6.5 (3.0-8.5) 

17 

6.2 (5.0-9.0) 16 

6.5 (5.1-9.0) 24 


a Summary statistics (mean, observed range in parentheses, and sample size) for measurements of USNM 338726, 
446481, 446482, 483363, 483364. 
b USNM 483359 (holotype), 483365. 

c Summary statistics (mean, observed range in parentheses, and sample size) for measurements of AMNH 209358, 
273093, 273126, 278465, 278500; CEBIOMAS 100; MUSM 863, 5589, 5932, 13205, 15209, 21173, 24350 (holotype); 
USNM 530962, 549362, 549363, 584475. 

d Summary statistics (mean, observed range in parentheses, and sample size) for measurements of AMNH 273069, 
273124; CEBIOMAS 101; MUSM 5523, 5541, 5542, 5933, 5940, 15207, 15208, 15210, 31927-31930; USNM 530960, 
530961, 549364, 584474. 

e Summary statistics (mean, observed range in parentheses, and sample size) for measurements of FMNH 87070; 
MUSM 21172; USNM 335180, 393014, 407797-407799, 407802, 460097, 528325, 549366, 549367, 574511, 575486, 
575488, 575497, 582300, 582301. 

f Summary statistics (mean, observed range in parentheses, and sample size) for measurements of AMNH 16120 (holo¬ 
type), 267940, 267943; MUSM 5509, 5931, 21170, 21171; USNM 306582, 361570, 361571, 385753, 393013, 407796, 
407801, 407803, 415387, 415388, 456537, 460098, 530958, 530959, 549369, 559186, 560560, 574510, 575489-575491, 
575493, 575494, 575496, 575498, 582299. 


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c 


FIGURE 4. Occlusal views of partial upper toothrows in Hsunycteris dashe (A, MUSM 15206), H. pattoni (B, 
MUSM 13205), and H. thomasi (C, AMNH 16120) illustrating taxonomic differences in the morphology of 
the premolars and first molar (see text). Abbreviations: p, parastyle of Ml; P4, first upper premolar; P5, sec¬ 
ond upper premolar; Ml, first upper molar. 

metacarpal V is longer than metacarpal IV in H. dashe, whereas metacarpal V is shorter than IV 
in H. cadenai and H. pattoni, and these metacarpals are subequal in length in H. thomasi. 

The skull of Hsunycteris dashe is distinguished from those of all other species in the genus 
by having a relatively broader rostrum and lacking inflation of the postorbital region (versus 
rostrum narrower and postorbital region inflated in H. cadenai, H. pattoni, and H. thomasi). 
The postorbital region lacks a lateral projection in H. dashe, H. pattoni, and H. thomasi, whereas 
a lateral projection is present in H. cadenai (see Woodman and Timm, 2006: fig. 11 A). The 
lateral margin of the infraorbital foramen does not project beyond rostral outline in dorsal view 
in H. dashe, whereas the infraorbital foramen is wider with a lateral margin that projects 
beyond rostral outline in dorsal view in H. cadenai, H. pattoni, and H. thomasi. The sphenoidal 
crest is well developed in H. dashe, whereas this crest is weakly developed in H. cadenai, H. 
pattoni, and H. thomasi. The septum separating the left and right basisphenoid pits is narrow 
in H. dashe and H. pattoni, whereas the septum is broader in H. cadenai. 4 The maxilla imme- 


4 Hsunycteris thomasi exhibits considerable intraspecific variation in this feature, with some specimens having 
a relatively narrow septum (e.g., AMNH 267940) and others having a broader septum (e.g., AMNH 16120). 


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AMERICAN MUSEUM NOVITATES 


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diately posterior to M3 is less than the length of M3 in H. dashe, H. cadenai, and H. pattoni ; 
in contrast, the maxilla posterior to M3 is longer than the length of M3 in H. thomasi. 

The body of the dentary is deep in Hsunycteris dashe, H. cadenai, and H. thomasi, whereas 
it is shallow and the entire dentary appears more slender in H. pattoni. The coronoid process 
is low (extending dorsally slightly above the level of the articular condyle) in H. dashe and 
H. thomasi, whereas the coronoid process is significantly higher in H. cadenai and H. pattoni. 
The angular process is broad in H. dashe, H. cadenai, and H. thomasi, whereas it is narrower 
in H. pattoni. 

In lateral view, the inner and outer upper incisors are not in contact in Hsunycteris dashe, 
whereas these teeth are in contact in H. cadenai and H. pattoni (Hsunycteris thomasi exhibits 
variation in this character: the inner and outer upper incisors are in contact in some specimens 
[e.g., AMNH 16120] but not in others [e.g., AMNH 267940, 267943]). The outer upper incisors 
are large (slightly smaller than inner upper incisors) in H. dashe whereas they are proportionally 
smaller (less than half the size of the inner upper incisors) in H. cadenai, H. thomasi, and H. pat¬ 
toni. Whereas P4 lacks a lingual cusp in H. dashe (fig. 4A), H. cadenai, and H. pattoni (fig. 4B), 
this cusp is present in H. thomasi (fig. 4C). The lingual cusp of P5 is weakly developed in H. dashe 
(fig. 4A), whereas this cusp is well developed and narrow in H. pattoni (fig. 4B) and well devel¬ 
oped and broad in H. cadenai and H. thomasi (fig. 4C). There is a small gap present between P5 
and Ml in H. dashe, H. cadenai, and H. pattoni, whereas this gap is variable H. thomasi (e.g., 
present and wide in AMNH 16120, but absent in AMNH 267940 and 267943). The parastyle on 
Ml is well developed and labially oriented in H. dashe. In contrast, the parastyle is weakly devel¬ 
oped and directed anteriorly in H. cadenai, while it is well developed and directed anteriorly in 
H. pattoni and H. thomasi. The protocone basins of Ml and M2 are broad in H. dashe and H. 
thomasi, whereas they are reduced in H. cadenai and H. pattoni. The third upper molar is large 
in H. dashe, H. cadenai, H. pattoni, and some specimens of H. thomasi (e.g., AMNH 267940, 
267943), whereas other specimens of H. thomasi have smaller M3s (e.g., AMNH 16120). 

The lower incisors are large and mesiodistally broad in Hsunycteris dashe and H. cadenai, 
whereas these teeth are proportionally smaller and narrower in H. thomasi and H. pattoni. The 
distal cusp on pi is weakly developed in H. dashe, whereas it is well developed in H. cadenai, 
H. pattoni, and H. thomasi. The anterior cusp of p4 is oriented horizontally in H. dashe, whereas 
this cusp in H. cadenai and H. pattoni is inclined upwards. Hsunycteris thomasi exhibits intra¬ 
specific variation in this feature, with some individuals having the cusp oriented horizontally 
(e.g., AMNH 267940, 267943) while it is inclined upwards in others (e.g., AMNH 16120). The 
paracristid notch of ml is strongly developed in H. dashe and H. cadenai, but this notch is 
weakly developed or absent in H. pattoni and H. thomasi. The hypoconid of m2 is wide in H. 
dashe and H. cadenai, whereas it is narrow in H. thomasi and H. pattoni. 

Morphometric Analyses: Our multivariate statistical analysis included only female speci¬ 
mens because males are unknown for Hsunycteris dashe. We compared three specimens of H. 
cadenai, 14 of H. pattoni, 18 of H. thomasi, and two of H. dashe (appendix 1), using a principal 
components analysis (PCA) based on one external measurement (FA) and the 11 craniodental 
measurements described above. The first three principal components accounted for 82.4% of the 


PC 3 (11.1%) PC 2 (14.9%) 


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15 


A 

0.15 

0.10 

0.05 

0.00 

-0.05 

- 0.10 

-0.15 

-0.20 -0.15 -0.10 -0.05 0.00 0.05 0.10 0.15 

PC 1 (56.3%) 

0.15 

0.12 

0.09 

0.06 

0.03 

0.00 

-0.03 

-0.06 


* * 

• 

• 

• 

O O 

• 


o 

A O 

O 

o 

o 

o 

o 0 

o • 

• 

° o 

° o • 

-0.20 -0.15 -0.10 

-0.05 

0.00 0.05 0.10 0.15 


PC 1 (56.3%) 


A Hsunycteris cadenai 
-*• H. dashe 
• H. pattoni 
O H. thomasi 


O A ° 

O 


O 

O 


FIGURE 5. Results of principal components analysis, illustrating the dispersion of specimen scores for female 
Hsunycteris cadenai (open triangles), H. dashe (asterisk), H. pattoni (filled circles), and H. thomasi (open 
circles). See text for explanation and appendix 3 for factor loadings and other results. 


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AMERICAN MUSEUM NOVITATES 


NO. 3881 


H. pattoni 


0.04 

Substitutions/site 


H. thomasi A 


L. orienticolina 


L. concava 


■ TK 104054 


G. soricina 


► L. handleyi 

rom 105786 —► L. chocoana 

TK 104602 
TK 104612 
TK 104601 
TK 135677 

lsumzm92i —► /_. hesperia 

TK 22549 I L ' s P urrel1 ' 

TK 22540 

tk 161667 -► P. genovensium 

mvz 186020 —►X. vierai 


FIGURE 6. Cytochrome-^ maximum likelihood (ML) phylogram for the subfamily Lonchophyllinae. Support 
statistics from ML analysis and Bayesian inference (BI) are indicated at each resolved node. For the ML analy¬ 
sis, gray shading indicates bootstrap frequencies between 50% and 75% and black indicates bootstrap frequen¬ 
cies >75%. For the BA, gray indicates posterior probabilities <0.95, whereas black indicates posterior 
probabilities >0.95. 

total variance in the log-transformed measurements of this material (appendix 3). PC 1 accounted 
for the highest percentage (56.3%), and this vector has uniformly positive loadings, suggesting 
that it is a size factor (with a notably high loading for coronoid height). Although all four species 
show overlapping scores on PCI and PC2 (fig. 5A), H. dashe specimens are widely separately 
from the other three species on PC3 (fig. 5B). Factor loadings on PC3 suggest that this separation 
is attributable primarily to differences in forearm length, width at canines, and width at M2. 


2017 


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Molecular Analyses: Molecular analysis of 
mitochondrial Cyt-b sequences from selected 
specimens (table 1) recovered well-supported 
clades consistent with the divergence of Hsunycte¬ 
ris from other lonchophyllines (fig. 6). The mono- 
phyly of Hsunycteris is strongly supported by these 
data, and H. dashe was recovered as the sister lin¬ 
eage of a robustly supported clade comprised of 
H. cadenai, H. pattoni, and H. thomasi in both 
Bayesian inference and ML analyses. Pairwise 
genetic comparisons between H. dashe and other 
congeneric species averaged at least 11% and 15% 
for uncorrected-p and K2P distances, respectively 
(appendix 4). 

Natural History: Our three specimens of 
Hsunycteris dashe were all collected at diurnal 
roosts discovered by Matses hunters near Nuevo 
San Juan. The first to be collected (MUSM 15206, 
an adult female) was found roosting alone beneath 
the undercut bank of a small stream in dense val¬ 
ley-bottom primary forest on 2 September 1999. 

D.W.F. collected this bat after having been led to the 
roost by the hunters who found it. According to his 
field notes, “the roof of the [undercut] bank was 
held together by the root mass of a nearby tree,” and 
the bat was hanging from this root-stabilized surface, about 1 m above the waters edge. The other 
two specimens (AMNH 273165, MUSM 15211; mother and young, respectively) were found 
roosting together with a third individual (which escaped capture) beneath the undercut bank of 
another stream, in primary upland forest on 21 October 1999. No additional details were pro¬ 
vided by the Matses hunters who collected these two specimens and described their roost to 
D.W.F. 

Except for the narrow floodplain of the Rio Galvez, the landscape surrounding Nuevo San 
Juan consists of low hills and terraces (nowhere more than 200 m above sea level) eroded from 
Miocene lake sediments; there are no caves or rock outcrops anywhere in the region. As 
described elsewhere, the average annual rainfall is probably close to 3000 mm. Except where 
cleared for Matses horticulture or regenerating from their slash-and-burn clearings, the local 
vegetation consists of a variety of primary formations determined by drainage and seasonal 
flooding (Fleck and Harder, 2000; Voss and Fleck, 2011). All our specimens of Hsunycteris 
dashe were taken in tall, undisturbed forest on hilly interfluvial terrain far from the palm 
swamps and seasonally flooded formations of the Galvez floodplain. 


FIGURE 7. Dashe, the Matses hero who led his 
people to victory in their struggle for survival dur¬ 
ing the mid-20th century. (Photographed by Ste¬ 
ven Romanoff on the upper Chobayacu, ca. 1975.) 


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AMERICAN MUSEUM NOVITATES 


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Etymology: For Dashe (ca. 1910-1980, fig. 7), also known as Quioshash, a hero of the 
Matses people. Dashe grew up during the rubber boom, when mercenaries were sent to Matses 
territory to exterminate the indigenous inhabitants. Dashe grew up fleeing from attackers who 
killed his kinsmen and carried off women and children to be prostituted or sold as slaves. After 
he had grown to manhood, Dashe rallied the Matses to fight back, leading multiple successful 
raids on rubber camps and settlements, eventually expelling all outsiders (Jimenez Huanan et 
al., 2014). Without his courage and military cunning the Matses would no longer exist as an 
intact culture with legally recognized title to their tribal land. 


DISCUSSION 

With the description of Hsunycteris dashe the subfamily Lonchophyllinae now includes 20 
species grouped in five genera, three of which are monotypic (Parlos et al., 2014; Moratelli and 
Dias, 2015). The type locality of H. dashe (fig. 2: locality 35), is one of the most diverse sites in 
the Neotropics, with over 60 bat species documented to date (Fleck et al., 2002; Voss et al., 
2016). Only one other congener (H. pattoni) is known to occur at Nuevo San Juan, but a third 
species (H. thomasi ) has been recorded at Jenaro Herrera (fig. 2: locality 39), only 70 km to the 
northwest. Both of these localities lie within the Yavari-Ucayali interfluvial region. Accordingly, 
we expect that all three species (H. dashe, H. pattoni, and H. thomasi ) likely occur sympatrically 
in this part of northeastern Peru. By contrast, H. cadenai is (insofar as known) a Trans-Andean 
species that is unlikely to occur with H. dashe (see Mantilla-Meluk et al., 2010). 

The paraphyletic status of Hsunycteris thomasi was first reported by Parlos et al. (2014). 
Mitochondrial and nuclear markers support the grouping of H. thomasi specimens in two 
clades, one of which is more closely related to H. pattoni than the other (fig. 6). Confusingly, 
representatives of both clades of H. thomasi have been collected near the Venezuelan type 
locality (Parlos et al., 2014). In our morphological analyses we were unable to identify any 
morphological traits that unambiguously distinguish members of the two clades of H. thomasi 
recovered in our molecular analysis. To identify which of the two clades the name H. thomasi 
properly applies to, and which represents an undescribed taxon, we attempted to obtain 
sequence data from the holotype (AMNH 16120), a specimen that was collected in 1909. 
Unfortunately, our attempts to amplify mitochondrial fragments from the holotype have thus 
far been unsuccessful. 


Key to the Species of Hsunycteris 

1. Forearm > 35.0 mm; hairs between the shoulders >9 mm; dermal papillae on chin arranged 
in a V and separated by a wide basal cleft; metacarpal V longer than metacarpal IV; ros¬ 
trum broad; lateral margin of infraorbital foramen does not project beyond rostral outline 

in dorsal view; outer upper incisors large; P5 lingual cusp weakly developed. 

. Hsunycteris dashe 


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VELAZCO ET AL.: NEW SPECIES OF HSUNYCTERIS 


19 


1'. Forearm <34.5 mm; hairs between the shoulders <8 mm; dermal papillae on chin 
arranged in a V but not separated by a wide basal cleft; metacarpal V shorter than or 
subequal to metacarpal IV; rostrum narrow; lateral margin of infraorbital foramen does 
project beyond rostral outline in dorsal view; outer upper incisors small; P5 lingual cusp 
well-developed.2 

2. Postorbital region with a lateral projection; Ml parastyle weakly developed; lower incisors 

large and broad; ml paracristid notch strongly developed; m2 hypoconid wide. 

. Hsunycteris cadenai 

2'. Postorbital region lacks a lateral projection; Ml parastyle well developed; lower incisors 
small and narrow; ml paracristid notch weakly developed or absent; m2 hypoconid 
narrow.3 

3. Metacarpal V shorter than metacarpal IV; extent of maxillary posterior to M3 less than the 

length of M3; dentary slender; angular process narrow; P4 lingual cusp absent; P5 lingual 

cusp narrow. Hsunycteris pattoni 

3'. Metacarpal V subequal to metacarpal IV; extent of maxillary posterior to M3 greater than 
the length of M3; dentary deep; angular process broad; P4 lingual cusp present; P5 lingual 
cusp broad. Hsunycteris thomasi 


ACKNOWLEDGMENTS 

We are grateful to our Matses hosts and field assistants at Nuevo San Juan, where R.S.V. 
and D.W.F. collected bats in 1998 and 1999; to the Institute Nacional de Recursos Naturales 
(INRENA), which issued the necessary collecting and export permits; and to the MUSM (espe¬ 
cially Victor Pacheco and Sergio Solari), which provided important logistical support in Lima. 
Our 1998/1999 field research at Nuevo San Juan was partially supported by grants from the 
AMNH Center for Biodiversity and Conservation. The following curators and collection staff 
graciously provided access to specimens under their care: Erika Paliza (CEBIOMAS); Bruce 
Patterson (FMNH), Victor Pacheco (MUSM); and Alfred Gardner, Darrin Lunde, and Suzanne 
Peurach (USNM). Alfred Gardner and an anonymous reviewer provided helpful comments on 
the submitted draft of this manuscript. Patricia J. Wynne drew figures 2, 3, and 4. Alejandra 
Camacho provided information about Ecuadorean coordinates. We thank Steven Romanoff for 
permission to reproduce his photograph of Dashe. 


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APPENDIX 1 
Specimens Examined 

The following list includes all specimens used in the morphological components of this 
study with data on their respective localities. See Material and Methods for abbreviations. 
Coordinates are provided in appendix 2. Specimens used in the morphometric analyses are 
marked with an asterisk. 

Hsunycteris cadenai (N = 7). COLOMBIA— Valle del Cauca : Bajo Calima, ca. 45 km by air 
NNE of Buenaventura, along the Rio Calima (USNM 338726*); across from the Village of 
Zabaletas, east bank Rio Zabaleta, 29 km SE Buenaventura (USNM 446481, 446482, 483359 
[holotype], 483363*, 483364*, 483365). 

Hsunycteris dashe (N = 3). PERU— Loreto: Alto Amazonas, Nuevo San Juan, Galvez River 
(AMNH 273165*; MUSM 15206* [holotype], 15211). 

Hsunycterispattoni (N = 37). BOLIVIA— Beni: 1.5 km below Costa Marquez, Itenez River 
(AMNH 209358*). Santa Cruz: Parque Nacional Kempff Mercado, Meseta de Huanchaca, 
Huanchaca I (USNM 584474, 584475*). BRAZIL— Amazonas: 80 km N by road of Manaus 
(USNM 530960, 530961, 530962*). Para: Altamira, 52 km SSW, E Bank Rio Xingu (USNM 
549362*, 549363*, 549364). PERU— Loreto: Alto Amazonas, Nuevo San Juan, Galvez River 
(AMNH 273069, 273093, 273124-273126; MUSM 13205*, 15207-15210); Maynas, Punchana, 
Barrio Orosa Estacion Madreselva II, Rio Amazonas (MUSM 31927-31930); Quebrada Blanco, 
Comunidad de Limon (MUSM 21173*); Requena, Jenaro Herrera, Centro de Investigaciones 
Jenaro Herrera (AMNH 278465*, 278500*; CEBIOMAS 100*, 101; MUSM 863*, 5523, 5541, 
5542, 5589*, 5932*, 5933, 5940). Madre de Dios: Tambopata, north bank of the Rio Madre de 
Dios, 14 km E Puerto Maldonado, Reserva Cuzco Amazonico (MUSM 24350* [holotype]). 

Hsunycteris thomasi (N = 55). BRAZIL— Amazonas: 80 km N by road of Manaus (USNM 
530959); Manaus, University (USNM 530958). Para: Altamira, 52 km SSW, E Bank Rio Xingu 
(USNM 549366*, 549367*, 549369); Belem, Fazenda Velha (USNM 361570, 361571); Belem, 
Mocambo (Igapo) (USNM 393013, 393014*); Belem, Utinga (USNM 460098); Belem, Varzea 
(USNM 460097*). ECUADOR— Napo: Rio Yasuni (USNM 528325*). Pastaza: Tiguino, 130 km S 
of Coca (USNM 574510, 574511*). FRENCH GUIANA— Cayenne: Paracou, near Sinnamary 
(AMNH 266106, 266110, 267451,267451, 267940, 267943). GUYANA— Barima-Waini: Baramita 
(USNM 582299, 582300*, 582301*). PANAMA— Bocas del Toro: Nuri (USNM 575486*, 575488*, 
575489-575491, 575493, 575494, 575496, 575497*, 575498). Darien: mouth of Rio Paya (USNM 
306582). San Bias: Armila, Quebrada Venado (USNM 335180*). PERU— Loreto: Maynas, Rio 
Maniti, Santa Cecilia (FMNH 87070*); Quebrada Blanco, Comunidad de Limon (MUSM 21170, 
21171,21172*); Requena, Jenaro Herrera, Centro de Investigaciones Jenaro Herrera (MUSM 5509, 
5931). VENEZUELA— Amazonas: Capibara, 106 km SW Esmeralda, Brazo Casiquiare (USNM 


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415387); Casiquare Canal, Capibara (USNM 415388); Cerro Neblina Base Camp, Rio Mawarinuma 
(USNM 559186); Puerto Ayacucho, 32 km S Puerto Ayacucho, Raya (USNM 407802*, 407803); 
San Carlos de Rio Negro, ca 7 km E (USNM 560560); San Juan, 163 km ESE Puerto Ayacucho, 
Rio Manapiare (USNM 407798*, 407799*, 407801); Tamatama, Rio Orinoco (USNM 407796, 
407797*). Bolivar: Ciudad Bolivar (AMNH 16120 [holotype]); El Manaco, 59 km SE El Dorado, 
km 74 (USNM 385753); Icabaru, 45 km NE Icabaru, Santa Lucia de Surukun (USNM 456537). 


APPENDIX 2 

Gazetteer of Collecting Localities 

Below we list the localities of all the specimens and/or tissues used in this study. Names of 
the largest administrative unit (department, state, etc.) within each country are italicized, and 
geographic coordinates are provided. 

BOLIVIA 

1. Beni, 1.5 km below Costa Marques (-12.4833, -64.3000). 

2. Santa Cruz, Parque Nacional Kempff Mercado, Meseta de Huanchaca, Huanchaca I 

(-13.9075, -60.8147). 

BRAZIL 

3. Amazonas, 80 km N by road of Manaus (-2.4000, -59.7167). 

4. Amazonas, Manaus, University (-3.1333, -60.0166). 

5. Para, Altamira, 52 km SSW, E Bank Rio Xingu (-3.6500, -52.3700). 

6. Para, Belem, Fazenda Velha (-1.4500, -48.4833). 

7. Para, Belem, Mocambo (Igapo) (-1.4500, -48.4833). 

8. Para, Belem, Utinga (-1.4500, -48.4833). 

9. Para, Belem, Varzea (-1.4500, -48.4833). 

10. Paraiba, Fazenda Espirito Santo, near Campina Grande, Municipio de Soledade (-7.0833, 

-36.3500). 

COLOMBIA 

11. Valle del Cauca, Bajo Calima, ca. 45 km by air NNE of Buenaventura, along the Rio Calima 

(4.0167, -77.0000). 

12. Valle del Cauca, across from the Village of Zabaletas, east bank Rio Zabaleta, 29 km SE 

Buenaventura (3.7333, -76.9500). 

ECUADOR 

13 Esmeraldas, 2 km S Alto Tambo (0.9216, -78.5500). 

14. Esmeraldas, Comuna San Francisco de Bogota (1.0935, -78.7059). 

15. Esmeraldas, Terrenos Aledanos de la Comuna San Francisco de Bogota (ca. 1.0935, 

-78.7059). 


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16. Esmeraldas, E San Lorenzo, banana plantation (1.2586, -78.7808). 

17. Esmeraldas, E San Lorenzo, La Guarapera farm and pasture (1.2702, -78.8030). 

18. Esmeraldas, San Jose Farm, E San Lorenzo towards Lita (1.0100, -78.6222). 

19. Morona Santiago, Huamboya, Cueva de los Tayos, por el rio Paztaza (-1.936432, -77.793260). 

20. Napo, Rio Yasuni (-0.9300, -75.9500). 

21. Pastaza, 5 km E Puyo, Safari Hosteria Park (-1.7333, -78.0000). 

22. Pastaza, Puyo, Finca el Pigual (-1.4797, -77.9966). 

23. Pastaza, Tiguino, 130 km S of Coca (-1.1167, -76.9500). 

24. Pichincha, Mejia, La Union del Toachi, Otongachi (-0.313829, -78.9544). 

FRENCH GUIANA 

25. Cayenne, Paracou, near Sinnamary (5.2833, -52.9167). 

GUYANA 

26. Barima-Waini, Baramita (7.3714, -60.4958). 

27. Potaro-Siparuni, Iwokrama Reserve, 5 km SW of Kurupukari, Giadonda Camp (4.6333, 

-58.7167). 

PANAMA 

28. Bocas del Toro, Nuri (8.9167, -81.8167). 

29. Darien, Cana (7.7833, -77.7000). 

30. Darien, mouth of Rio Paya (7.9167, -77.5167). 

31. San Bias, Armila, Quebrada Venado (8.6667, -77.4500). 

PERU 

32. Arequipa, 2 km NE of Atiquipa, “El Castillo,” (-15.7811, -74.3476). 

33. Huanuco, 6 km N Tingo Maria (-9.2336, -75.9833). 

34. Lambayeque, Las Juntas, in Quebrada La Pachinga, ca. 14 km N, 25 km E Olmos (-6.4500, 

-79.8667). 

35. Loreto, Alto Amazonas, Nuevo San Juan, Galvez River (-5.2500, -73.1667). 

36. Loreto, Maynas, Punchana, Barrio Orosa Estacion Madreselva II, Rio Amazonas (-3.6277, 

-72.2401). 

37. Loreto, Maynas, Rio Maniti, Santa Cecilia (-3.5555, -72.8833). 

38. Loreto, Quebrada Blanco, Comunidad de Limon (ca. -4.3166, -73.2333). 

39. Loreto, Requena, Jenaro Herrera, Centro de Investigaciones Jenaro Herrera (-4.8986, 

-73.6503). 

40. Loreto, San Jacinto (-2.31667, -74.86667). 

41. 4Madre de Dios, Hacienda Erika, Rio Alto Madre de Dios opposite Salvacion (-12.8491, 

-71.3876). 

42. Madre de Dios, Tambopata, north bank of the Rio Madre de Dios, 14 km E Puerto Maldo¬ 

nado, Reserva Cuzco Amazonico (-12.5500, -69.0500). 


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SURINAM 

43. Brokopondo, Brownsberg Nature Park, 8 km S, 2 km W of Brownsweg (4.9167, -55.1667). 

44. Brokopondo, Marowijne, 3 km SW of Albina (5.4667, -54.0833). 

45. Nickerie, Bitagron (Kayserberg Airstrip) (3.1000, -56.4667). 

VENEZUELA 

46. Amazonas, Capibara, 106 km SW Esmeralda, Brazo Casiquiare (2.6200, -66.3200). 

47. Amazonas, Casiquiare Canal, Capibara (2.6167, -66.3167). 

48. Amazonas, Cerro Neblina Base Camp, Rio Mawarinuma (0.8300, -66.1700). 

49. Amazonas, Puerto Ayacucho, 32 km S Puerto Ayacucho, Raya (5.4000, -67.6500). 

50. Amazonas, San Carlos de Rio Negro, ca 7 km E (1.9167, -67.0667). 

51. Amazonas, San Juan, 163 km ESE Puerto Ayacucho, Rio Manapiare (5.3000, -66.2200). 

52. Amazonas, Tamatama, Rio Orinoco (3.1700, -65.8200). 

53. Bolivar, Ciudad Bolivar (8.1333, -63.5500). 

54. Bolivar, El Manaco, 59 km SE El Dorado, Km 74 (6.2800, -61.3200). 

55. Bolivar, Icabaru, 45 km NE Icabaru, Santa Lucia de Surukun (4.5500, -61.4200). 

56. Bolivar, Rio Grande, 28 km E El Palmar (8.0067, -61.6972). 


APPENDIX 3 

Principal Component Factor Loadings 

Loadings for the first three factors extracted from a principal components 
analysis of 12 measurement variables. See Material and Methods for definitions and 

abbreviations of variables. 


Measurements 

PC 1 

PC 2 

PC 3 

FA 

0.100 

0.052 

0.511 

GLS 

0.228 

0.028 

-0.158 

CIL 

0.259 

0.138 

-0.141 

CCL 

0.260 

0.173 

-0.101 

BB 

0.188 

-0.117 

0.161 

C-C 

0.302 

-0.243 

0.424 

MPW 

0.260 

0.055 

0.241 

MTRL 

0.263 

0.480 

-0.183 

M2-M2 

0.190 

0.219 

0.534 

DENL 

0.268 

0.209 

-0.125 

MANDL 

0.252 

0.463 

-0.090 

COH 

0.608 

-0.579 

-0.280 

Proportion of variance (%) 

56.3 

14.9 

11.1 


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APPENDIX 4 

Matrix of Genetic Distances 

Average percent uncorrected (p) and Kimura 2-parameter (K2P) genetic distances for 
Hsunycteris species estimated using the R package ape v4.1. All sequences were cropped 
to the first 400 bp of the mitochondrial Cyt-b gene. Uncorrected-p distances shown 
below the diagonal and K2P distances shown above the diagonal. Values along the 
diagonal represent within group K2P pairwise distances for each Hsunycteris group. 


1 

2 

3 

4 

5 

1. H. cadenai 

0.5 

14.0 

13.4 

13.4 

11.4 

2. H. dashe 

12.4 

- 

12.2 

15.0 

12.8 

3. H. pattoni 

11.9 

10.9 

1.8 

7.9 

8.5 

4. H. thomasi A 

13.2 

13.2 

7.4 

0.3 

8.1 

5. H. thomasi B 

11.4 

11.4 

5.2 

7.6 

2.3 


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