TF-IUPS160013 81..95


REVIEW ARTICLE

Pancreatic islet blood flow and its measurement

Leif Janssona, Andreea Barbua, Birgitta Bodina, Carl Johan Drotta, Daniel Espesa,b, Xiang Gaoa, Liza Grapensparra,
€Orjan K€allskoga, Joey Laua, Hanna Liljeb€acka, Fredrik Palma, My Quacha, Monica Sandberga, Victoria Str€omberga,
Sara Ullstena and Per-Ola Carlssona,b

aDepartment of Medical Cell Biology, Uppsala University, Uppsala, Sweden; bDepartment of Medical Sciences, Uppsala University, Uppsala,
Sweden

ABSTRACT
Pancreatic islets are richly vascularized, and islet blood vessels are uniquely adapted to maintain and
support the internal milieu of the islets favoring normal endocrine function. Islet blood flow is normally
very high compared with that to the exocrine pancreas and is autonomously regulated through com-
plex interactions between the nervous system, metabolites from insulin secreting b-cells, endothelium-
derived mediators, and hormones. The islet blood flow is normally coupled to the needs for insulin
release and is usually disturbed during glucose intolerance and overt diabetes. The present review pro-
vides a brief background on islet vascular function and especially focuses on available techniques to
measure islet blood perfusion. The gold standard for islet blood flow measurements in experimental
animals is the microsphere technique, and its advantages and disadvantages will be discussed. In
humans there are still no methods to measure islet blood flow selectively, but new developments in
radiological techniques hold great hopes for the future.

ARTICLE HISTORY
Received 3 March 2016
Accepted 8 March 2016

KEYWORDS
Blood flow measurements;
islet blood flow;
microspheres; pancreatic
islets

In 1960 Claes Hellerstr€om and co-workers published a paper
in which they tried to assess the b-cell activity by quantifying
the number of erythrocytes in the islets (1). A correlation
between islet endocrine activity and blood flow was assumed,
but this was difficult to demonstrate due to lack of precision
in the method. He did not, however, forget the topic, and
20 years later in 1980 one of the authors (L.J.) of the present
review began studying the islet vasculature under the ben-
evolent and extremely stimulating guidance of Claes.

Claes, you were, as always, correct! There is a correlation
between islet endocrine activity and blood flow, and you
helped to develop this field of research. We aim to give a
brief overview of the islet vasculature, and focus on the
methods that can be used to measure its blood flow, discus-
sing the advantages and disadvantages with the various
techniques.

1. Pancreatic islet morphology

A. Cellular composition

In’t Veld and Marichal have provided an excellent overview of
pancreatic islet morphology (2) where further references can
be found. In most vertebrates pancreatic islets are distributed
throughout the pancreas in cellular aggregates containing
from a few up to several thousands of cells. They are demar-
cated by a connective tissue capsule, the extent of which is
species-dependent. Most focus on islet function has been
directed towards their endocrine cells, in particular the insu-
lin-producing b-cells. These cells constitute 40%–70% of all

endocrine cells in the islets, depending on species. Common
laboratory animals, i.e. mice and rats, have more b-cells
(60%–70%) than humans (40%–50%) (3). The other islet endo-
crine cells are glucagon-producing a-cells, somatostatin-pro-
ducing d-cells, pancreatic polypeptide-producing PP-cells, and
ghrelin-producing e-cells. Most islets contain a mixture of
these cells. A notable exception is the uneven distribution of
PP- and a-cells, where the former are found mainly in the
caput region, i.e. the former embryonic ventral anlage,
whereas a-cells are found mainly in the tail region, corre-
sponding to the dorsal anlage. b-Cells are more evenly dis-
tributed in the pancreas, even though humans seem to
possess occasional b-cell-rare islets. It should be noted that
smaller islets contain predominantly b-cells, whilst the other
endocrine cell types are mainly found in the larger islets.

The reasons for the coexistence of these hormone-produc-
ing cells in discrete micro-organs are not known for certain
(4), and we will briefly return to this issue later, since we
believe that this organization profoundly affects the interac-
tions between endocrine cells and islet vasculature to achieve
a fine-tuning of islet hormone release.

Besides the endocrine cells, the islets contain numerous
other cell types, vascular cells, other stromal cells, immune
cells, and neural elements (Table 1). The present review
focuses mainly on the blood perfusion of the islets, and we
will therefore discuss in more detail the cells associated with
the islet vasculature. Nervous elements in the islets consist of
nerve cells with axons, referred to as neuro-insular complexes
type 1 when there are nerve cells bodies, and type II when

CONTACT Leif Jansson, leif.jansson@mcb.uu.se Department of Medical Cell Biology, Biomedical Centre, Box 571, Husargatan 3, SE-75123 Uppsala, Sweden
� 2016 Informa UK Limited, trading as Taylor & Francis Group. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creative-
commons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited

UPSALA JOURNAL OF MEDICAL SCIENCES, 2016
VOL. 121, NO. 2, 81–95
http://dx.doi.org/10.3109/03009734.2016.1164769



only intra-islet axons are found (5,6). Many of these nerves
affect not only hormones secretion per se, but also islet blood
flow. The Schwann cells should be mentioned in this context,
since they seem to surround all islets in an envelope, but
their functions remain enigmatic (7). It has been suggested
that they may participate in regenerative processes after islet
transplantation (8).

Immune cells can be numerous during islet inflammations,
i.e. insulitis, but are normally sparse in the islets. Interestingly,
it has recently been suggested that recruitment of different
subtypes of macrophages may influence the vascularization
of islets, especially after transplantation (9,10). However, these
notions are beyond the scope of this review.

Among stromal cells fibroblasts contribute by forming the
thin network of reticular and collagenous fibers in the islets
as well as the capsule surrounding each islet. Normally also
pancreatic stellate cells with their characteristic lipid droplets
can be seen (11). Their exact function in the islets is
unknown, but their numbers are increased during desmoplas-
tic reactions to pancreatic adenocarcinomas as well as during
chronic pancreatitis (12). In both these instances they contrib-
ute to the pancreatic fibrosis characteristic of these condi-
tions. We have also noted that their numbers in islets are
increased in GK rats, a type 2 diabetes model characterized
by islet fibrosis (11). There are myofibroblasts present under
these conditions as well (13), but whether they emanate from
the stellate cells or other cell types is unknown. Another stro-
mal cell in islets is the interstitial cell of Cajal, a cell of neural
origin. Such cells are common in the intestine where they
serve as pacemaker cells, being active in regulation of intes-
tinal motility (13). Whether such effects occur also in the pan-
creas is an intriguing possibility, but so far unknown (14).

B. Morphology of pancreatic islet vasculature

This subject has been highlighted in several reviews
(2,15–21). The islets contain fenestrated capillaries, which

constitute 8%–10% of the islet volume, and are organized
into a glomerular-like network, described already in the 1880s
(22), i.e. at a time when islet function was unknown. The
number of fenestrae is approximately 10 times higher than in
exocrine pancreatic capillaries (23) and is induced by the high
local production of vascular endothelial growth factor-A
(VEGF-A) from the islet b-cells (24,25). Thus, after transplant-
ation when islets are implanted into organs with continuous
capillaries, the ingrowing new microvessels initially form such
capillaries, but already after a few days the endothelium
becomes fenestrated (26). It is likely that the fenestrations
facilitate hormonal passage into the circulation as well as par-
ticipate in draining extracellular fluid analogous to functions
normally performed by lymphatic capillaries (27). Besides
being fenestrated, islet capillaries are wider than those in the
exocrine pancreas, having a 20%–30% larger diameter, and
their vascular density is much higher (23). It can be noted
that after transplantation the vascular density of the islet
grafts in sites such as the liver is less than that in endogen-
ous islets for several months post-transplantation (15,28).

Pericytes located between the endothelium and the capil-
lary basement membrane can occasionally be found, but they
are not particularly numerous (8,29). Their functions in islets
are little studied and largely unknown. It has been hypothe-
sized that they contribute to angiogenesis or as contractile
cells (8), but these notions are mainly conjectural.

The larger islets contain one to three afferent arterioles,
which originally branch from intralobular arteries in the exo-
crine tissue. These afferent arterioles sometimes contribute
tributaries also to exocrine acini, but many of them supply
only the islets (16). Smaller islets are directly incorporated
into the capillary network of the exocrine pancreas. The
organization of larger islets means that there is an anatomical
correlate, which enables autonomic regulation of the islet
blood perfusion. The diameter of the afferent arteriole is usu-
ally 20–30 lm (Figure 1), and it contains one, or occasionally
two, layers of vascular smooth muscle cells (VSMC), which are
surrounded by adventitial tissue containing fibroblasts, but
also occasional adipocytes (30).

The anatomy of the veins draining the islets is to some
extent species-dependent and also depends on the size of
the islets. As mentioned above, smaller islets drain with exo-
crine veins, whereas larger islets have a different organization
(16). Most common is a direct venous drainage to one to four
larger veins with a basket-like network of smaller vessels lying

EXOC

EXOCRINE PANCREAS

Blood flow: 0.4-1.0 ml/min x g

PO2: 40 mmHg

Capillary pressure: 6-7 mmHg

Blood flow: 5-6 
ml/min x g

PO2: 40 mmHg

Capillary pressure: 
4-5 mmHg

ISLET

Figure 1. Blood flow values in exocrine and endocrine pancreatic parenchyma.
Modified from Jansson and Carlsson (15).

Table 1. Cell types in pancreatic islets.

Cell types

Endocrine cells a-cells
b-cells
d-cells
e-cells
PP-cells

Stromal cells Fibroblasts
Myofibroblasts
Stellate cells
Cajal cells
Occasional duct cells

Vascular cells Endothelial cells
Vascular smooth muscle cells
Pericytes
Adventitial stromal cells

Immune cells Granulocytes
Lymphocytes
Macrophages
Dendritic cells
Mast cells

Neural cells Neurons
Schwann cells

Data from (2,20).

82 L. JANSSON ET AL.



in association with the connective tissue capsule at the inter-
face between the islets and the surrounding exocrine tissue.
These veins then empty into intralobular veins and, finally,
into the portal vein. However, some of the islets, particularly
in larger mammals, have a so-called insulo-acinar portal sys-
tem. This means that the islet capillaries empty into numer-
ous small venulae, which then anastomose with capillaries in
the exocrine pancreas. By such means there are two serially
connected capillary systems, i.e. a portal system. In rodents
this is of minor importance, but its role in human islets, as
well as other primates, is likely to be larger even though this
is little studied (16,31).

In general, islets are devoid of lymphatic capillaries,
whereas the exocrine pancreas contains numerous such ves-
sels (27,32). Lymphatics draining the pancreas contain insulin,
but at a concentration <30% of that seen in the portal vein
(33). To what extent this represents recirculation of insulin is
unknown. In islet grafts, lymphatics initially develop, but with
time they decline in number (34). These findings have been
interpreted to reflect that the highly permeable islet blood
capillaries, as well as the small size of the islets, preclude the
need for lymphatic drainage. Other endocrine organs, such as
the pituitary and parathyroid glands contain lymphatics, but
they are much larger than those of islets, and the need to
prevent prolonged release of hormones into the circulation
by the lymphatics is not present. From an evolutionary point
of view, the Brockman bodies seen in fish, i.e. centimeter-
large accumulations of islet tissue, contain lymphatics (35).

2. Functional implications of islet morphology on
blood flow regulation

All functional evidence suggests that islet blood flow is regu-
lated autonomously from that of the exocrine pancreas and
that this regulation occurs at a pre-capillary level, i.e. in the
arteriole (36); for a summary see Brunicardi et al. (21,37).
There is no evidence that post-capillary regulation located to
the draining veins occurs (38). In this section we will provide
a more detailed overview of the sites that we believe are of
importance for islet blood flow regulation.

A. Arterioles

The presence of VSMC in the arterioles provides the basis for
the separate regulation of islet blood flow. Both arterioles
and the endocrine cells themselves receive efferent nerves,
particularly sympathetic nerve fibers, but also non-adrenergic,
non-cholinergic (NANC) nerves (5,6,39). The latter are presum-
ably purinergic and/or nitric oxide (NO)-containing nerves
(40). Furthermore, afferent sensory nerves affecting blood per-
fusion (41) can also be found within the islets (42). A sum-
mary of the effects of nerves on islet blood flow and insulin
secretion is provided in Table 2.

Arteriolar VSMC are also responsive to most locally pro-
duced endothelium-derived vasoactive substances but can be
affected by substances, including hormones, reaching them
through the systemic circulation as well. Islet endothelium,
mainly in arterioles but also capillaries, produces both NO

and endothelin-1 (30,43) and probably several other media-
tors that may directly influence the VSMC. The prime import-
ance of NO for islet blood regulation has been repeatedly
demonstrated (44,45).

During the last few years, increased focus has been
directed against the adventitia of resistance vessels, since e.g.
adipocytes, macrophages, and other cells found here may
also produce substances, such as adipokines, cytokines, and
gaseous transmitters, which may affect VSMC through intra-
vessel paracrine mechanisms. We have for instance observed
that GK rats, a type 2 diabetes (T2D) model, express more
interleukin-6 in their adventitia than normal rats (unpublished
observation). A further influence on arteriolar VSMC may be
derived from substances produced by adjacent endocrine
cells. It should be noted that some arterioles branch at the
periphery of the islets, whilst others penetrate into the islet
core before forming into capillaries (16,37,46). This means
that a variable part of the arteriole is exposed to high con-
centrations of substances produced within the islets. These
substances include islet hormones and factors co-released
with endocrine granules, e.g. chromogranins, synaptophysins,
and Zn2þ (47). Furthermore, other substances produced by
metabolically active endocrine cells, namely nucleotides such
as ATP, ADP, and adenosine, may also be present in high con-
centrations close to the VSMC (48). It is easy to envisage that
such substances may affect both endothelial cells and VSMC
in the arterioles and thereby affect blood flow. However, to
what extent they may also affect ionic channels in capillary
endothelial cells and then transmit retrograde signals to the
arterioles (49) is an intriguing concept, but one not yet fully
explored.

B. Capillaries

Since capillaries consist of a tube of single endothelial cells
surrounded by a basement membrane, they do not in general
possess any blood flow regulatory properties. No signs of any
pre-capillary sphincters have been noted in either islet arterio-
les or proximal capillaries, so it seems likely that the flow
regulation is indeed mainly restricted to the arterioles. There
are occasional pericytes (29,50), but their contractility and par-
ticipation in flow regulation in mammals are controversial.

Morphological studies of islet capillaries, as well as studies
on isolated islet endothelial cells, have not demonstrated any

Table 2. Effects of different neurotransmitter
substances on insulin release and islet blood
flow (IBF).

Insulin IBF

Muscarinic (M3) receptors þ þa
b1 Adrenoceptors 0 0
b2 Adrenoceptors þ –
b3 Adrenoceptors 0 þb
a1 Adrenoceptors – þ
a2 Adrenoceptors 0 0

b

D2 receptors – þb
D3 receptors 0 0

Data from (5,95,166,167).
aInhibitory effect during hyperlipidemia.
bNormalizes increased basal islet blood flow in

GK rats, a type 2 diabetes model.

UPSALA JOURNAL OF MEDICAL SCIENCES 83



heterogeneity between individual islets. The organization of
the islet capillaries is usually described as glomerulus-like, and
islets are highly vascular, although not as profound in human
as in rodent islets (51,52). Most b-cells have at least parts of
their cytoplasm facing a capillary, and the endocrine granules
are preferentially located in this part of the cytoplasm (53).
This seems to be the case also for the other islet endocrine
cells, with the possible exception of d-cells. The latter cell
type contains long, slender processes which establish contact
with other cell types and to some extent also to the islet
capillaries (54).

This endocrine cell polarity provides the basis for the B-A-
D flow hypothesis formed on morphological observations and
perfusion studies in rodent islets, but has also been sug-
gested to be valid for human islets (55). Rodent islets have a
b-cell-rich core surrounded by a mantle of non-b-cells. The
arterioles are described as entering the islets through a dis-
continuity in this mantle, and then branch into capillaries in
the b-cell-rich core of the islets (Figure 2). This would mean
that high local insulin concentrations are transported in the
blood towards the periphery of the islets, where a-cells would
add glucagon and, finally, the d-cells their somatostatin.
Paracrine/endocrine interactions between the islet endocrine
cells are thereby, at least partially, mediated by the flow dir-
ection in the islets (56). Besides these morphological studies,
also functional studies with retrograde perfusions corroborat-
ing these notions have been performed (55). It is worthy of
note, however, that this theory has been disputed (21).
Indeed, there have also been suggestions that the blood flow
direction instead is from the periphery towards the center or
from ‘top to bottom’ without any direct correlate to micro-
regions of different endocrine cells (21,37). In an elegant
study Nyman and co-workers (46) examined this in detail in
mice and found that all of these patterns could be found, but
that core-to-mantle constituted approximately 50% of the
studied islets. For technical reasons these studies were

confined to larger islets. We have in a series of experiments
in rats retrogradely injected microspheres and confirmed the
findings of Nyman and co-workers (unpublished
observations).

C. Veins

The morphology of the venous drainage has been mentioned
in the preceding section. The morphology of the veins them-
selves is similar to that of other veins and venulae in the
body, and as expected no valves have been described.
Venous VSMC are sparse, and the vessel size is quite variable.
Venulae associated with insulo-acinar portal systems are small
and have a diameter of only 15–20 lm (57). There is no evi-
dence of any flow control by the activity of venular VSMC
(38). An interesting observation is that when islets are trans-
planted the graft is drained exclusively by larger veins, and
no signs of an insulo-acinar portal system can be discerned
(58). Another issue of importance is that islet inflammation,
such as insulitis, which is associated with a mononuclear cel-
lular infiltration, seems to be initiated in the islet periphery
(59,60), i.e. at the location of the veins. In the diabetes-prone
BioBreeding/Worcester rat, an animal model of type 1 dia-
betes, an islet venular defect has also been described (61).
Moreover, occasional mast cells, which affect venular perme-
ability, can be found at this location (62), and the number of
mast cells is increased in T2D (63). After islet transplantation,
so-called ‘blood lakes’ are formed, which probably emanate
from disrupted veins. They restitute and become replaced by
connective tissue a few days post-transplantation (15).

D. Islet cellular composition affecting vascular
morphology

The islet vascular architecture referred to above is probably
not static, but is likely to vary not only between different
islets but also over time and depending upon the functional
demands on the endocrine cells (64). It has been known that
smaller islets in rodents with diameters <100 lm mainly con-
tain b-cells (65). These islets seem to be incorporated into the
exocrine capillary system (66). This implies that the regulation
of islet blood flow in smaller islets is probably not autonomic
from that of the exocrine pancreas, but is regulated in con-
cert with the latter. It should be noted, however, that the
contribution of the smaller islets to the total pancreatic islet
volume is small (65), so a majority of islet endocrine cells are
located to islets with an autonomous blood flow regulation.
Human islets sometimes consist of many a-cells, but the
blood flow regulation of such islets is at present unknown.
An interesting comparative physiological approach in this
context is that some birds, e.g. ducks, have islets containing
predominantly a-cells, and the vasculature of such islets dif-
fers from that of b-cell-containing islets (67).

Another factor which affects not only the cellular compos-
ition per se but also islet blood flow is age. Before birth islets
are small and very few islet capillaries have developed, but in
the post-partum period islet endocrine and vascular mass
both rapidly expand (68). Nevertheless, the blood perfusion

Figure 2. Estimation of intra-islet insulin concentrations based on previously
published data on insulin release (168) and islet blood flow (87).

84 L. JANSSON ET AL.



in 5-week-old animals is considerably lower than in older
animals. For instance, the fractional islet blood flow in
5-week-old rats is only 1%–2%, which increases to 8%–10%
after 15 weeks, 15% after 12 months, and >20% at 2 years of
age (69–71). Similar findings have been made in mice (72).
This increase is present also when adjusted for changes in
islet volume. We believe that this reflects increased insulin
resistance with age, but the exact mechanisms behind the
increase are not known, even though it seems likely that NO
is involved (73).

When islet growth is stimulated as after partial pancreatec-
tomy (74,75) and during pregnancy (76) there is usually an
increased islet blood perfusion. A controversial issue in the
context of islet growth is to what extent new islets may form
by ‘budding’ from precursor cells in smaller pancreatic ducts,
an issue previously taken for granted (77,78), but lately
refuted (79). There are some older studies suggesting that
peri-ductular islets derive their arterial blood from ductal
blood vessels (80), and it has even been suggested that duc-
tal blood vessels constitute a third capillary network in an
intra-pancreatic portal system (81). In that latter study the
authors described that the first system would be in islets, the
second in exocrine tissue, and, as mentioned, a third in ducts.
Such islets would probably contribute very little to total islet
volume, and therefore be of little importance.

E. Pancreatic blood flow and heterogeneity between
islets

When referring to blood flow values in the exocrine and
endocrine pancreas we use values obtained by the micro-
sphere technique. The blood perfusion of the pancreatic islets
is considerably higher than that of the exocrine gland, and it
is, in adult rats, 5%–20% of total pancreatic blood, despite
the islet volume constituting only 1%–2% of the pancreas.
Normally, there is a close correlation between islet blood flow
and total pancreatic blood flow (Figure 3), but during e.g.
hyperglycemia their responses become dissociated (82,83).
When correcting for weight, the corresponding value for islet
blood flow is 5–6 mL/min�g islets (Figure 1), which is one of

the higher blood flow values in the body, normally only sur-
passed by that to the oxygen-sensing glomus cells in the
carotid body (84). Very high flow values were recorded also
in other species such as for instance Atlantic hagfish (85),
mouse (86), and rabbit (87). There are, however, no differen-
ces in blood perfusion between islets in the head region of
the gland, i.e. pancreatic polypeptide-rich islets supplied by
the superior mesenteric artery, and those in the tail region
which are glucagon-rich and receive their blood from the
celiac trunk (88). This holds true for the exocrine pancreas as
well, which despite its dual arterial supply regulates its blood
flow synchronously (89).

Of interest in this context is whether this high blood
perfusion involves all islets, or only some of them, which
would then constitute an extremely well-perfused and pre-
sumably functionally more active subgroup. Indeed,
repeated microsphere injections have indicated that micro-
spheres predominantly end up in the same 10% of islets
(90), and that these islets further increase their blood perfu-
sion in response to glucose (90). Injection of a marker of
low oxygenation, pimonidazole, demonstrated that
20%–25% of the islets are normally poorly oxygenated and
with less protein biosynthesis than others, but become bet-
ter oxygenized at increasing demands for insulin release
(28). With a keen eye to its limitations the microsphere
technique has been used to identify tentatively the most
highly perfused islets, and differences in vascular density,
glucose metabolism, b-cell proliferation, and insulin release
have been identified, suggesting that there is indeed a
coupling between islet blood flow and metabolic activity
(91,92). It is worthy of note, however, that only insulin has
been studied in this context, and it is unknown if such
relationships exist also for other islet hormones. The obser-
vation of a highly perfused subgroup of islets opens the
intriguing notion that islets receiving lower blood flow may
constitute a functional reserve, which can increase their
flow and thereby their functional activity upon demand. It
is tempting to speculate that this may be a safety measure
to prevent an excessive insulin release at any given time. It
would also provide a twist to the question raised for many
years (4), why b-cells are distributed into a vast number of
tiny cell aggregates rather than forming a large, compact
gland like most other endocrine organs.

3. Techniques used to study islet blood flow

The high islet blood flow is normally further increased when-
ever there is a need for increased insulin secretion, and this is
assured by complex interactions between several regulatory
mechanisms. Furthermore, conditions with decreased glucose
tolerance, when there is a need for augmented insulin
release, are also associated with an increased islet blood flow
(89), and such factors ensuring these blood flow responses
include:

1. Metabolic factors from b-cells: We have noted that
especially adenosine and ADP seems to be of major
importance for this, and directly couple the degree of

IBF (µl/min x g pancreas)

10 20 30 40 50 60 70

P
B

F
 (

m
l/m

in
 x

 g
)

0,0

0,2

0,4

0,6

0,8

1,0

1,2

Figure 3. Correlation between islet blood flow (IBF) and total pancreatic blood
flow (PBF) on anesthetized normoglycemic Sprague-Dawley rats. Data are based
on 36 recent control experiments. (Pancreatic blood flow ¼0.0466þ (0.0158 �
islet blood flow)). P < 0.001.

UPSALA JOURNAL OF MEDICAL SCIENCES 85



metabolism to the required blood flow increase
(93,94).

2. Nervous system: The vagus nerve, sympathetic nerves,
and sensory nerves all affect islet blood flow, and their
effects are summarized in Table 2 (95).

3. Endothelium-derived constricting and dilating factors: So
far approximately 10 different substances in this category
have been examined, and the responses are as expected.
The pronounced sensitivity for NO shows its major
importance for islet blood flow regulation (44).

4. Hormones: Islet hormones, incretins, and adipokines are
potential regulators of islet blood flow. With the excep-
tion of incretin hormones, there are only sparse effects
of hormones on islet blood flow, but incretins seem to
potentiate glucose-induced stimulation of islet blood
flow (96).

These blood flow regulatory mechanisms are very similar
to those mediating responses also in other tissues, and espe-
cially so to those mediating postprandial reactive hyperemia
in the gut (97). However, with regard to the islets it seems as
if the major factor affecting islet blood flow is the prevalent
blood glucose concentration, and this may be by activating
one or several of the factors referred to above (83,90,98). This
would then modulate the blood perfusion according to the
needs of the insulin-secreting b-cells. To the best of our
knowledge there is no similar coupling between the release
of the other islet hormones and blood flow.

The distribution of the islets within the exocrine paren-
chyma means that measurements of total pancreatic blood
flow is not sufficient, since the fraction of the blood flow
being diverted to the islets is unknown. Therefore, measure-
ments must separately register endocrine and exocrine blood
flow. This precludes the use of several common methods
used to assess regional blood circulation, such as those based
on the Fick principle, or electro-magnetic or ultrasound flow
probes placed around arteries or veins in the organ. These
techniques can only determine total pancreatic blood flow,
and since the pancreas has multiple arterial supplies, both
the superior mesenteric artery and the celiac trunk, this
necessitates the placement of at least two probes (89). Also
techniques based on radiological methods such as magnetic
resonance imaging (MRI) and positron emission tomography
(PET), which have the added benefit of being applicable to
humans, provide measurements only of total pancreatic blood
flow, mainly due to the fact that the resolution is not suffi-
ciently high to allow visualization of individual islets.
However, these problems are at present being overcome, and
in the foreseeable future radiological techniques may allow
visualization of the islet organ to allow not only determina-
tions of islet blood perfusion, but even more importantly to
quantify islet mass in patients (99). Several techniques have
been experimentally applied to assess islet blood flow, almost
exclusively in rodents and mainly in rats. The predominant
techniques that have been used to investigate the blood per-
fusion of endogenous islets are different in vivo microscopy
applications, microsphere measurements, and most recently
hydrogen gas clearance. Studies on transplanted islets have

applied mainly in vivo microscopy and laser-Doppler flowme-
try, but also microspheres have been tried (15,100). We will
now comment on advantages and disadvantages with these
techniques with a major focus on measurements in endogen-
ous islets.

A. Microsphere measurements of islet blood flow

This technique is a variant of the deposition techniques (see
below under D). Then, instead of chemical substances, small
polystyrene particles (commonly referred to as microspheres)
are injected into the arterial blood stream. They are distrib-
uted into the different capillary beds, where they become
entrapped. In this manner, nutritive blood perfusion rather
than plasma perfusion is measured, since the microspheres
distribute as erythrocytes. The number of microspheres within
each organ is proportional to their blood perfusion, and this
can be assessed by quantification of their numbers, either dir-
ectly by counting or by assessing their labels, which can be
radioactivity, fluorescence, or different colors (101).

The first experiments applying entrapped particles to
measure local blood flow were carried out with starch par-
ticles in pigs (102), but other materials such as ceramics have
been used. The technique in its present form was introduced
in 1967, when isotope-labeled plastic particles with a diam-
eter of 50 lm were injected into fetal lambs (102). This dem-
onstrated that, in comparison with antipyrine measurements,
these microspheres did not recirculate to any significant
extent, distributed in proportion to the blood flow, and did
not affect the circulation physiology in the fetuses, i.e. fulfilled
the basic criteria of the microsphere technique. The year after,
the concept of an arterial reference sample had been intro-
duced (103), which made measurements of cardiac output
with this technique possible. Since then this application has
developed into the gold standard for regional and intra-organ
blood flow measurements (101,104–106).

The adequate use of microspheres necessitates the fulfill-
ment of several criteria, namely: 1) Adequate mixing of the
microspheres with blood in the central circulation; 2)
Complete extraction of microspheres during the first passage
through the tissues; 3) Flow properties similar to those of red
cells; 4) No circulatory artifacts should be induced by the
microspheres; 5) The microspheres (or their marker if they are
labeled with something) should remain in the tissues; and 6)
The measuring accuracy should be sufficient.

Most islet blood flow studies, which were first performed
in the early 1980s (71,83,87) have used polystyrene plastic
particles with a diameter of 10 lm (or occasionally 15 lm)
stained black or other colors. Fluorescence-labeled micro-
spheres have been used as well (91,92), whilst microspheres
with radioactive tracers have been rarely used, even though
they have been commonly utilized for measurements of other
organ blood flow values (107).

(i) Criteria for the adequate use of microspheres. It is import-
ant that the microspheres are adequately mixed with the
arterial circulation and occupy the entire vessel profile, so
that their disposal into the tissues mimics that of red blood
cells. This can most easily be achieved by administering the

86 L. JANSSON ET AL.



microspheres where arterial blood flow is turbulent, i.e. into
the left atrium or ventricle or in the ascending aorta. Indeed,
the heart is the only choice if myocardial blood flow is to be
studied, since the coronary arteries branch immediately above
the aortic valves. In studies in rats less variation in the flow
determinations were seen after intra-atrial injections (108).

However, in small animals such as rats and mice cannula-
tion of especially the left atrium, but also the left ventricle,
can be difficult. An alternative experimental maneuver may
be to give the microspheres via cardiac puncture, an
approach chosen in Mongolian gerbils (109). The placement
of the catheter within the heart can be determined by pres-
sure recordings during catheter insertion. There is, however,
always a risk of complications by e.g. damage to the aortic
valves, since the catheters used for microsphere injections
should not be too thin. A diameter of 1 mm is usually
required in order to avoid impaction of the microspheres. We
usually give the injections into the ascending aorta. We
advance the catheter down to the plane of the aortic valves,
which can be felt, and then withdraw it 1–2 mm. At this site
there is no interference with aortic flow or cardiac output.
Furthermore, the precision of blood flow determinations in
the pancreas is similar as when applying intraventricular
microsphere injections (110). As a rule of thumb intra-aortic
microsphere injections provide adequate precision for blood
flow determinations in organs below the diaphragm, whereas
for organs above the diaphragm administration into the heart
is necessary.

Another prerequisite for adequate mixing is that the
microspheres do not adhere to one another and form larger
aggregates in the microcirculation corresponding to large
chains of microspheres. The latter was observed in some ini-
tial studies where microsphere behavior in the hamster cheek
pouch microcirculation was studied with intravital microscopy
(111). Formation of such aggregates or chains is prevented
today by addition of Tween to the microsphere solutions.

In all experiments applying microspheres it is desirable to
investigate the microsphere content in paired organs, such as
the kidneys or adrenal glands. Since we count the micro-
spheres in a microscope (see below) we prefer the latter for
logistic reasons, i.e. there is a smaller number of microspheres
to count. The number of microspheres found is usually in the
order of >500 per gland, and this should not differ by more
than 10% between the glands if adequate mixing has
occurred.

(ii) Complete extraction during first passing. This is of utmost
importance, since recirculation of the microspheres will pro-
vide erroneous results, with overestimations of blood flow in
well-perfused organs. To avoid this, the microspheres should
have a size which is larger than the smallest arterioles and
capillaries of the organ. Initial studies of microspheres in gen-
eral led to the conclusion that 15 lm microspheres should be
chosen, since their general systemic shunting is small. It has
also been shown that the distribution of microspheres of this
size correlates well with the distribution of labeled red blood
cells (112).

Thus, to minimize shunting of microspheres through capil-
laries of an organ, a microsphere size as large as possible
should preferentially be used. However, this imposes some

problems. Firstly, it is advantageous to have as many micro-
spheres as possible within the sample to increase the accuracy
of the flow measurement (113). Furthermore, smaller micro-
spheres end up in smaller arterioles/metarterioles and thereby
increase the resolution of the flow measurement (83). Many
studies on microsphere shunting are from the early days of
microsphere usage. These batches were very variable with
regard to size; for instance 15 lm microspheres were actually
in the range of 15 ± 5 lm (mean ± standard deviation), and
even larger size heterogeneity occurred. The result of this was
that there was a predominance of larger microspheres in the
peripheral tissues, whilst the smaller sizes recirculated. This
would of course produce errors especially with regard to intra-
organ flow distribution (104). At present microsphere batches
are much more homogeneous, and those with a diameter of
10 lm have a standard deviation of approximately 0.2 lm.

A simple way of assessing the total degree of shunting of
microspheres in the whole body is to measure the amount of
microspheres in the lungs. The normal bronchial circulation is
<1% of cardiac output, so microspheres exceeding that
amount in the lungs represent microspheres shunted in the
periphery. With the use of 10 lm microspheres in rats,
approximately 2% of the injected microspheres are found at
this location (110). In the whole vascularly perfused pancreas
approximately 3%–4% of the microspheres enter the portal
vein (114). Granted, this is in the whole pancreas, and we do
not know for sure whether there are any direct shunts
through the islets. There are anecdotic reports that this may
occur (100). However, no reports from in vivo microscopy of
islets have described any shunting of microspheres through
or around the islets. In this context we would like to stress
that, as outlined in the next section, the microspheres are
supposed to mimic red cells, i.e. produce a measure of nutri-
tive blood flow. If there is shunting allowing red cells to
bypass the islets, it still means that the microspheres measure
the nutritive blood flow.

(iii) Flow properties similar to those of red blood cells. An
issue of importance in this context is so-called ‘skimming’ of
microspheres. This was originally described in kidneys, where
microspheres traveled centrally in interlobular arteries, and
thereby erroneously preferentially accumulated in the outer
regions of the cortex (115,116). This is also referred to as
steric restriction affecting the distribution of the micro-
spheres. If considering the vascular anatomy in the pancreas,
this seems unlikely to occur in this organ, and skimming is
not of importance for most organs in the body.

The microsphere size we prefer to use, i.e. 10 lm, is similar
to the diameter of red cells. The likelihood of skimming
increases with size (115), as well as the simple fact that micro-
spheres become too large to enter some arterioles if they are
large enough. Islet arterioles are usually 30 lm (30), and we
have indeed noted a decreased islet blood flow if micro-
sphere size is increased (83). The question is in which arteri-
olar size microspheres of different diameter become
entrapped. Initial studies with in vivo microscopy of hamster
cheek pouches and bat wings demonstrated that the arterio-
les with impacted microspheres were surprisingly large,
namely in the order of 20–60 lm (111,117,118). It was also
noted that some 10 lm microspheres could slip through the

UPSALA JOURNAL OF MEDICAL SCIENCES 87



capillaries (118). When examining rodent pancreases injected
with ink, it seems as if 10 lm microspheres will be found in
islet arterioles of a size only marginally larger than the micro-
spheres themselves. When microspheres of different sizes
were used to determine arteriolar size, there were some
uncertainties in the precision of these estimates (119). For
reasons provided below, we believe that designed islet micro-
spheres are representative of islet blood perfusion per se, and
do not represent microspheres that have erroneously entered
islet capillaries.

(iv) On circulatory artifacts induced by microspheres. Major
factors to take into account in this context are the number
and size of the injected microspheres. The microspheres that
become entrapped in the regional vascular beds act as
emboli. This means that, depending on their number and
location, they may induce local ischemia and disturb both the
microcirculation as well as the general circulation. The num-
ber of microspheres that can be injected without causing any
undue effects on circulation has been the subject of numer-
ous studies in the past (101,105,113). However, since the size
uniformity of microsphere batches has improved markedly in
recent years, with absence of erroneously large microspheres,
many previously encountered problems have diminished. In
early studies of the microsphere technique a total number
varying between 60,000 and 320,000 15 lm and 10 lm micro-
spheres, respectively, was reported not to induce any hemo-
dynamic disturbances in rats (120,121). Occasionally, but not
always, more than one million 10 lm microspheres could be
given without adverse effects (121). We are consistently
injecting 300,000 microspheres with a diameter of 10 lm in
300-g rats and 100,000 in mice without ever observing any
hemodynamic instability.

It is, however, essential to monitor basal circulatory param-
eters and blood gases to detect circulatory alterations. We
have evaluated the pancreas and islets microscopically for
signs of necrosis caused by embolizing microspheres without
noticing any such signs. However, if the number of injected
microspheres exceeded one million there was some exocrine
ischemic damage, whilst the islets remained unaffected
(unpublished observations).

It is also relevant to discuss the number of microspheres
needed to attain statistical precision in microsphere measure-
ments of blood flow, especially in smaller organs such as
islets or organs with low blood perfusion. In a seminal paper
in this context it was found that the number of microspheres
within organs followed a Poisson distribution (113). By apply-
ing statistical calculations they determined that in order to
obtain a 10% precision in their measurements, all samples, i.e.
arterial reference sample and organ samples, should contain
at least 384 microspheres (113). This topic has been an issue
of much debate (149,150), and the consensus today is that
the experimental error can be kept as low as 10%–15% also
with a substantially lower number of microspheres in the
samples. It was shown empirically in rats that this was
the case when samples contained 200 microspheres (122).
The application of the technique to ocular structures and the
cochlea led to considerably lower numbers of microspheres
in the tissue samples, but it was shown empirically and theor-
etically that the errors in the determinations still remained

low (123,124) provided that the flow values exceeded 10 lL/
min (125). In these instances as few microspheres as around
50 were sufficient.

When microsphere measurements of islet blood flow were
initially performed, these issues were discussed in detail
(71,83,87,126). When applying the microsphere technique in
rats the reference sample contains >2,000 microspheres,
whereas the whole pancreas contains 2,000 microspheres and
the islets 200–400 depending on the experimental manipula-
tions. Note that the microsphere content in all islets is sum-
marized and the islets are considered to be one organ. The
flow value to the whole islet organ is in the order of
60–100 lL/min, i.e. well within the limits to achieve results
with statistical significance.

(v) Microspheres should be retained in the tissue. After injec-
tion the microspheres themselves are supposed to remain in
the tissue, and not move after their initial impaction.
Nevertheless, it might happen that microspheres leave the ori-
ginal organ of impact and move into the venous circulation,
i.e. a delayed shunting. These microspheres usually end up in
the lungs. By such means there is an underestimation of the
true organ blood flow. In most cases when one blood flow
measurement with microspheres is carried out, the organ is
removed quickly (within minutes) after the injection, meaning
that there is little time for any further movement to occur.
However, if repeated measurements are performed there is an
increased risk for this to occur. In the case that microspheres
have different labels to enable separation of different batches,
this at least makes it possible to compare this over time. Thus,
the differently labeled microspheres within the lungs provide
a measure of the degree of shunting of different microspheres
(90). We have performed studies in rodents where we have
injected three differently labeled microspheres (different col-
ors) (90). We found no differences in basal blood flow and
interpreted this to reflect that there is no real delayed shunt-
ing within the pancreas of rodents of 10 lm microspheres.
These experiments also lend support to the notion that no cir-
culatory artifacts are induced by 10 lm microspheres in the
used doses, even if administration is repeated.

Another issue which may lead to delayed shunting is if the
microspheres induce local ischemia in the tissue and thereby
damage the vasculature so they can dislodge from their site
of impaction. This has been described mainly for larger micro-
spheres. In the myocardium up to 20% of the microspheres
can escape, also through lymph (127,128). However, no signs
of ischemia have been detected in the pancreas after micro-
sphere injections in the doses we use in rodents.

Another, and potentially serious, source of error is the
movement of microspheres within the organ, leading to redis-
tribution with time between different compartments. Such a
redistribution occurs in the intestine, where microspheres ini-
tially trapped in submucous capillary plexa can move to more
distal mucosal capillaries (129,130). This is caused by diameter
changes in the blood vessels ante- or post-mortem. In both
these referred studies perfusion pressure was varied, e.g. by
administration of isoproterenol. Obviously, it is difficult to use
microspheres to quantitate the blood flow if capillary systems
are connected in series with one another. In the liver, micro-
spheres only allow for blood flow measurements in the

88 L. JANSSON ET AL.



hepatic artery and not that through the portal vein (97).
Similar difficulties are encountered also when measuring renal
medullary blood flow, where the microspheres end up in glo-
meruli since they precede the medullar vessels (131).

Islet capillaries are in parallel to those of the exocrine pan-
creas so this is not a problem for islet blood flow measure-
ments. However, the flow to the exocrine pancreas is
underestimated by microspheres, since some islets are part of
an insulo-acinar portal system (2), which means that pancre-
atic acini receiving their arterial blood from this system can-
not be measured with microspheres. The exact contribution
of the portal system to exocrine flow is unknown.

Extraction of microspheres within the tissue in proportion
to blood flow assumes that the arterioles and capillaries are
homogeneous with regard to diameter and do not contain any
major thoroughfare channels with much larger diameter than
the microspheres. If there are marked variations it may lead to
preferential shunting in parts of the tissue, and thereby under-
estimations of flow. This is the case for many malignant
tumors, which contain large and immature blood vessels,
which often shunt microspheres (132,133). Islets have a homo-
geneous capillary diameter, but it is usually larger than that of
exocrine capillaries (23), suggesting that islet microspheres
could move from the islets into acinar capillaries or veins.
Alternatively, microspheres in an afferent arteriole could
potentially move from the arteriole, which is at least partially
within exocrine tissue and into an islet. We have performed
experiments where we have artificially altered the blood pres-
sure, both in vivo within the autoregulatory capacity of islets
(i.e. 70–140 mmHg) (38) and in vitro with different perfusion
pressures (114), without observing any signs of this. Moreover,
we have measured blood flow in islet adenomas in MEN1-
knockout mice, but due to the considerations dealt with above
we chose to use hydrogen gas clearance instead (29).

The possibility of delayed shunting of microspheres
through an organ, in particular those with blood vessels with
varying diameters, presents certain difficulties in the use of
microspheres to assess organ blood flow. Thus, newly formed
blood vessels in islet grafts are initially immature with wide
diameter variations (26), leading to possible shunting or
movements of microspheres. The use of other techniques
such as laser-Doppler flowmetry (15) or hydrogen gas clear-
ance (134) is therefore highly warranted.

(vi) Measuring accuracy. This is mainly an issue when trac-
ers from the microspheres are extracted from the tissue of
interest. Microspheres can be purchased labeled with a radio-
active isotope, a fluorescent substance, or different colors
(101). Radioactivity can be measured with conventional tech-
niques, and as long as a whole organ is of interest there are
usually no problems, provided that the isotope is stably incor-
porated into the microspheres. Fluorescence or dyes can be
extracted from the organs of interest according to the manu-
facturer’s instructions, usually involving basic liquids, and then
quantified spectrophotometrically.

With regard to pancreatic islets there is an additional prob-
lem, which is that they constitute only 1%–2% of the pan-
creas. To quantify the number of microspheres within islets
we mainly rely on direct microscopic counting of the micro-
spheres. This can be done in histologic sections, but this is

extremely cumbersome. It has, though, been tried on islet
grafts (135). Since the microsphere diameter is fairly large,
there is always a risk that the microtome damages them and
thereby distorts the tissue architecture. When applying micro-
spheres to islet blood flow measurements, different ways to
clear the exocrine tissue (and thereby visualize both islets
and microspheres in thick sections) have been applied. We
have applied a freeze-thawing technique, which allows us to
quantify microspheres and their localization with a high
degree of certainty by manual counting (136,137). The islets
can usually be identified directly as whitish aggregates of
cells, and if stains such as neutral red or dithizone are
applied, their identity can be confirmed (71,137).
Alternatively, the pancreas can be cleared with e.g. methyl
salicylate or other substances (71,87,138). It is important to
ascertain that all microspheres have been visualized and that
intra-islet microspheres are identified with certainty. The cor-
relation between quantifications in cleared tissues and con-
ventional histological sections is excellent (110).

An alternative approach would be to isolate the islets with
collagenase and then count the number of microspheres
being present in the islets, as well as in the remains of the
digest. This has been tried, with radioactive microspheres, but
the results have been published only in abstract form (107).
The major problem with this approach is that only a limited
number of islets can be isolated with this technique, usually
in the order of 50%–60% of the larger islets, and none of the
smaller ones. This means that only a sample of the islets can
be used for the determinations, and since there is a hetero-
geneity in islet blood flow (vide supra) it is not known if this
sample is representative. Fluorescent microspheres have been
used, to isolate microsphere-containing islets, but in this con-
text the exact degree of islet recovery is unknown (91,92).

(vii) Use of microspheres for other purposes than blood flow
measurements. Microspheres can be impregnated with e.g.
cytostatic drugs or radioactivity and then injected into organs
where they become entrapped and then produce high local
concentrations of drugs or radioactivity. This approach has
especially been used to treat hepatic tumors since they
receive almost all their blood from the hepatic artery. If tribu-
taries to this artery are embolized with large microspheres—
often sizes of up to 50 lm have been used—the normal liver
parenchyma still receives sufficient oxygen and nutrients from
the portal vein to survive. Such microspheres can be made of
starch or albumin, or, in the case of radioactivity, yttrium-
labeled polystyrene (139). We have tentatively tried this
approach on islets implanted into the liver of mice. Such
derive their blood from the hepatic artery (140), and we
envisaged affecting islet graft cell replication. However, this
did not meet with any success (unpublished observation).
Since islet blood flow in the endogenous pancreas is much
higher than that to the exocrine pancreas, such an approach
would also be feasible for endogenous islets.

B. In vivo microscopy and pancreatic islet blood flow

By direct microscopic observations of islets, the earliest pub-
lished in 1882 by K€uhne and Lea, it has been possible not

UPSALA JOURNAL OF MEDICAL SCIENCES 89



only to map the vascular anatomy of the islets as outlined
above, but also to make direct observations on microcircula-
tion in islet capillaries (15,21,37,100). Confocal microscopy is
pivotal to the recent advances in this field, which allows for
visualization of the vascular architecture in thick sections and
whole islets. Furthermore, improved possibilities to stain islet
endothelial cells with different fluorescent antibodies and lec-
tins have contributed to the increased use of these techni-
ques (141). There are also transgenic mice whose islet
endothelial cells are spontaneously fluorescent (46).

One disadvantage with these techniques has been that
they are semi-quantitative. Possible ways to measure flow
include laser-Doppler velocimetry, which uses the frequency
shift produced by the Doppler effect when laser light is
reflected from moving blood cells (142). The direct calibration
of these values to blood flow is usually difficult to obtain,
whereas relative changes in flow can be easily monitored
(143). Another source of error when applying this technique
is that the penetration depth of the laser light into the tissue
needs to be evaluated, since blood cell movements in under-
lying tissues may otherwise disturb the measurements. So far
this technique has been applied mainly to transplanted pan-
creatic islets (15,100,144), since most of the laser probes are
too large to place over individual islets without undue distur-
bances from surrounding tissues.

Laser speckle is a random interference effect that gives a
grainy appearance to objects illuminated by laser light. If the
object consists of individual moving scatterers, such as blood
cells, the speckle pattern fluctuates. These fluctuations pro-
vide information about the velocity distribution of the scatter-
ers, i.e. blood cells (145). With the speckle technique it is also
possible to devise a full-field technique that gives an instant-
aneous map of velocities in real time. This technique has
recently been applied to transplanted islets (146), but its full
potential has not yet been developed.

Another way to assess microvascular flow is the dual-slit
cross-correlation technique (147), measuring the time it takes
for a red blood cell to traverse from a pre-set point to
another, which has been applied to islet grafts (10,100).

The techniques referred to above are all excellent for eval-
uations of graft blood flow or in some cases determinations
of microcirculation in single islets. The great disadvantage is
that they do not provide blood flow measurements per gram
of organ weight for the whole islet organ. Because there are
heterogeneities in islet blood flow, single islet flow determin-
ation becomes sensitive to such random variations.

A more recent application where the use of in vivo
microscopy has been taken one step further is the migra-
tion of macrophages and polymorphic neutrophilic granulo-
cytes (PMN) into islets. This has been applied both to
transplanted islets and endogenous islets by Phillipson and
co-workers, and they have been able convincingly to dem-
onstrate that maintenance of normal islet vasculature and
presumably b-cell mass and development depend on this
(148–150). In view of the importance of inflammatory reac-
tions in both T1D and T2D the true potential of this tech-
nique in this context is really staggering. Further details on
the use of in vivo microscopy can be obtained elsewhere
(21,46,100,148,151).

C. Perfusion of isolated, single islets

This technique is based on microdissection of single islets, a
technique originally developed by Claes Hellerstr€om (152),
with their arteriolar supply intact. The islet can then be stabi-
lized with holding pipettes, while the arteriole is cannulated
with a custom-made glass pipette (30) as previously described
for renal glomeruli (153). Islets are placed in a chamber on a
stage of an inverted microscope where movement and
adjustment of concentric holding and perfusion pipettes can
be made (Figure 4A). The system is then perfused with buffer
through the arteriole, and perifused around the islets, at a
perfusion pressure of approximately 40 mmHg. The experi-
mental set-up allows clear visualization of the arteriole, with
its vascular smooth muscle, and measurements of contraction
or dilation of the blood vessel (Figure 4B). This enables direct
studies of the vascular reactivity of the arterioles, without any
confounding factors from other tissues. However, although
blood flow regulation of individual islets can be investigated
in a unique manner, it is not possible to perform any meas-
urements on islet blood flow.

D. Flow deposition techniques for studies of islet blood
flow

These techniques are based on administration of substances
which are deposited in a tissue or volume of tissue in propor-
tion to its blood flow. This necessitates the choice of appro-
priate substances, as well as the possibilities to detect these

holding pipette

islet

pipette

arteriole

endothelial lining

VSM

(A)

(B)

Figure 4. A: Pancreatic islet being perfused after cannulation with a glass pip-
ette. The islet has a diameter of 250 lm. B: A close-up of the arteriole showing
two rows of vascular smooth muscle. The diameter of the arteriole is 34 lm.

90 L. JANSSON ET AL.



substances in the tissues of interest. A major difficulty is often
the detection step, especially when small structures such as
endogenous islets are of interest. However, the detection is
non-invasive, which would be a major advantage. Another
possible source of error is the degree of extraction of the
tracer. If that is low, it means that the fractional extraction is
higher in organs with low flow. This was the case for the ini-
tially used tracers such as rubidium-86 and potassium
(131,154). Different substances labeled with technetium-99
(155) or xenon-133 (156) have been used as well. At least in
their present form the resolution of the detectors applied
with these techniques is not sufficient to resolve islet
blood flow.

One more possibility, which so far has not been used for
determinations of islet blood flow, is determinations of
14C-antipyrine or 125I-antipyrine in tissues. These substances
accumulate in cells in relation to their delivery through blood
and can then be determined autoradiographically. The reso-
lution is excellent, but only relative values of blood flow are
provided. Furthermore, the technique is very time-consuming
and labor-intense (116,157).

We recently adapted the hydrogen gas clearance tech-
nique to measure both endogenous and transplanted islet
blood flow (134). This gives the possibility accurately and
repeatedly to measure the blood flow to the same islet.
However, in order to perform the measurements thin plat-
inum-electrodes must be inserted into the islets. These elec-
trodes detect the hydrogen concentration in the tissue, and
we can then measure its outflow after loading the animal
with inhaled hydrogen. The outflow rate has been shown to
be proportional to the blood flow. The requirements of elec-
trode insertion limit the number of islets available for the
measurements to those that can be directly observed. To
increase this number we used duct-ligated rats. Ligation of
the pancreatic duct leads to exocrine atrophy, but does not
interfere with islet blood flow (158). These studies verified the
actual blood flow values obtained with other techniques in
endogenous and transplanted islets, and confirmed the het-
erogeneity of islet blood flow (134).

E. Radiological techniques to measure islet blood flow

Recent rapid advancements in MRI and PET techniques make
it likely that it will soon be possible to measure blood flow in
endogenous islets in humans. Indeed, a recent study from
Turku has demonstrated that some conclusions on islet blood
flow may be inferred from studies on pancreatic perfusion
(159,160). Most studies are variants of flow deposit techni-
ques, where different tracers have been applied, and conclu-
sions on islet blood perfusion are indirect. There has been
intense activity to identify optimal markers, and at present
there are several available, some based on serotonin
(161,162). Another potential application is the use of 18F-flu-
oro-2-deoxy-D-glucose as a marker of inflammation. Nuutila
and co-workers have shown that this substance is taken up in
islets in NOD mice (163) and also that this substance can be
used to detect inflammations in e.g. endocarditis (164). This
substance would then serve as an excellent marker for

insulitis, and such preliminary studies have been presented. In
a recent study on LADA patients scintigraphy utilizing inter-
leukin-2 radiolabeled with (99m)Tc ((99m)Tc-IL-2) was applied
to detect insulitis (165), a technique previously used to image
chronic inflammatory-mediated disorders.

4. Concluding remarks

Despite technical difficulties it is possible to determine islet
blood flow in experimental animals. However, at present
there is no method which allows for determinations of islet
blood flow in humans. The knowledge gained so far from
blood flow measurements in experimental animals has shown
that the islets possess a blood flow regulation which is inde-
pendent of that for the whole pancreas, and uniquely
adapted to the metabolic needs of the endocrine cells. The
pancreatic islet blood flow is 5–10 times higher than that of
the exocrine pancreas, and can be selectively enhanced
whenever the need for insulin secretion is increased. There is
also compelling evidence that islet blood perfusion is dis-
turbed during conditions with impaired glucose tolerance
and overt type 2 diabetes. At present much work is put into
efforts to determine whether blood perfusion disturbances
are of pathogenic importance for the development of dia-
betes, or whether it is secondary to the metabolic disturban-
ces within and outside of the islets.

Disclosure statement

The authors report no conflicts of interest.

Funding information

Own work referred to in the review has been supported by grants from
the Swedish Research Council, the Swedish Diabetes Foundation, the
Swedish Juvenile Diabetes Foundation, Diabetes Wellness Sverige, the
Novo Nordisk Foundation, the Juvenile Diabetes Research Foundation,
and the Family Ernfors Fund.

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UPSALA JOURNAL OF MEDICAL SCIENCES 95


	Pancreatic islet blood flow and its measurement
	Pancreatic islet morphology
	Cellular composition
	Morphology of pancreatic islet vasculature

	Functional implications of islet morphology on blood flow regulation
	Arterioles
	Capillaries
	Veins
	Islet cellular composition affecting vascular morphology
	Pancreatic blood flow and heterogeneity between islets

	Techniques used to study islet blood flow
	Microsphere measurements of islet blood flow
	In vivo microscopy and pancreatic islet blood flow
	Perfusion of isolated, single islets
	Flow deposition techniques for studies of islet blood flow
	Radiological techniques to measure islet blood flow

	Concluding remarks
	Disclosure statement
	Funding information
	References