AU637199B2

AU637199B2 - Method for treating intestinal diseases

Info

Publication number: AU637199B2
Application number: AU72262/91A
Authority: AU
Inventors: Francis John Ballard; Leanna Christine Read
Original assignee: Gropep Ltd
Current assignee: Novozymes Biopharma DK AS
Priority date: 1990-02-13
Filing date: 1991-01-30
Publication date: 1993-05-20
Anticipated expiration: 2011-01-30
Also published as: AU7226291A

Description

INTERNA

INTERNAI

OPI DATE 03/09/91 AOJP DATE 10/10/91 APPLN. ID 72262 91 PCT NUMBER PCT/AU91/00031 rREATY(PCT) (11) International Publication Number: WO 91/12018 (51) International Patent Classification 5 A61K 37/36 Al (43) International Publication Date: 22 August 1991 (22.08.91) (21) International Application Number: (22) International Filing Date: 3 Priority data: PJ 8586 13 Febru PCT/AU91/00031 0 January 1991 (30.01.91) ary 1990 (13.02.90) AU (81) Designated States: AT (European patent), AU, BE (European patent), CA, CH (European patent), DE (European patent), DK (European patent), ES (European pptent), FR (Eur 'pean patent), GB (European patent), GR (European patent), IT (European patent), JP, LU (European patent), NL (European patent), SE (European patent), US.

Published With international search report, 637 99 (71) Applicant (for all designated States exceot US): GROPEP PTY. LTD. [AU/AU]; 39 Winwood Street, Thebarton, S.A. 5031 (AU).

(72) Inventors; and Inventors/Applicants (for US only) BALLARD, Francis, John [AU/AU]; 23 Lowan Avenue, G!enalta, S.A. 5052 (AU) READ, Leanna, Christine [AU/AU]; 4/46 High Street, Kensington, S.A. 5068 (AU).

(74)Agent: PHILLIPS ORMONDE FITZPATRICK; 367 Collins Street, Melbourne, VIC 3000 (AU).

(54) Title: METHOD FOR TREATING INTESTINAL DISEASES (57) Abstract A method for the treatment of disorders in gut function in animals including humans, which method includes administering to a patient to be treated an effective amount of a mammalian insulin-like growth factor-I (IGF-I) or a peptide analogue thereof.

WO 91/12018 PCT/AU91/00031 -1- METHOD FOR TREATING INTESTINAL DISEASES This invention relates to insulin-like growth factor-I (IGF-I) and its analogues. More particularly, the invention relates to the use of IGF-I and its analogues to treat disorders in gut function, e.g.

relating to the effects of intestinal diseases.

IGF-I is a small protein that has been shown to stimulate the growth of cells in culture. Animal growth is also stimulated in pituitary-deficient, normal and catabolic states. Kidney function is also improved.

These studies have led to the interpretation that IGF-I may be usefully applied in humans: to treat growth hormone deficiencies; to suppress the loss of body protein in catabolic states following burns, infection or other trauma; and as a treatment for patients suffering from renal diseases.

A number of human diseases result either in the subject having a lesser amount of gut tissue than required for normal digestion or absorption, or alternatively a diseased but normal-length gut in which digestion or absorption is impaired. Examples of human diseases that fit these two categories include short-gut syndrome, chronic ulcerative gut diseases, inflammatory gut diseases such as colitis and Crohn' disease, and necrotising enterocolitis in infants.

IGF-I is not known in the prior art to increase the growth or function of the cell types that comprise the abdominal gut, viz the stomach, duodenum, jejunum, ileum, cecum and colon. It is these regions of the gut that are affected in the diseases described above. Gut tissues do contain receptors for IGF-I (for example see: M. Laburthe et al, Am. J. Phsyiol. 254, G457, 1988; D.J. Pillion et al., Am. J. Physiol. 257, E27, 1989; H. Werner et al, Proc. Natl. Acad. Sci. USA 86, 7451, 1989), and are known under certain conditions to synthesise IGF-I or IGF-I messenger RNA (for example see: P.K. Lund et al., J.

Biol Chem. 261, 14539, 1986; A.J. D'Ercole et al., WO 91/12018 PCT/AU91/00031 -2- Pediatr. Pe Z. 20 5, 253, 1986 h1.-A. HcU± IIL Histochemistry 89, 403, 1988; W.L. Lowe, Jr., J. Clin.

Invest. 84, 619, 1989).

IGF-I has previously been administered to dwarf mice, hypophysectomized rats, diabetic rats, starved mice and rats, normal rats, mini poodles and normal human subjects. The levels of IGF-I have also been increased by insertion of an IGF-I-expressing transgene in mice. In most of these studies IGF-I treatment has led to an increase in body growth. It has been noted that an undesirable side effect of high doses of IGF-I is hypoglycemia. However, in none of the reported studies was there any indication of an IGF-I effect on the abdominal gut. For example in one investigation where over expression of IGF-I was produced by transgenesis and led to substantial body growth in transgenic mice, the fractional weight of the duodenum was the same as in IGF-deficient animals Behringer et al., Endocrinology 127, 1033, 1990). In another study the administration of low doses of IGF-I to suckling rats did not alter the weights of gastrointestinal organs (G.P.

Young et al., Digestion 46S2, 240, 1990). In particular, there exists no prior report on the increase of gut weight following IGF-I administration.

It is accordingly an object of the present invention to overcome or at least alleviate, one or more of the difficulties related to the prior art.

The first aspect of the present method concerns the treatment of animals, including humans, with disorders in gut function by using mammalian, preferably human IGF-I.

Accordingly in a first aspect of the present invention there is provided a method for the treatment of disorders in gut function in animals, including humans, which method includes administering to a patient to be treated an effective amount of mammalian insulin-like growth factor-i (IGF-I) or a peptide analogue thereof.

herein, we mean disordras r one-or- more of the-stomach, duodenum7ojunum plu- ilcum,- and colon. Such-d'isorders This invention also provides a pharmaceutical or veterinary composition when used for the treatment of disorders in gut function, including an effective amount of a mammalian insulin-like growth factor-I or peptide analogue thereof; and a pharmaceutically or veterinarily acceptable diluent carrier or excipient therefor.

This invention further provides a method for the treatment of disorders in gut function, which method includes administering to a patient to be treated a pharmaceutical or veterinary composition including an effective amount of a mammalian insulin-like growth factor-I analogue thereof; and a pharmaceutically or veterinarily acceptable diluent carrier or excipient therefor intravenously, subcutaneously, intramuscularly or enterily at a dose rate of approximately to 5000 microgram/kg body weight/day for a period of approximately 1 to 6 days.

By the term "disorders in gut function", as used herein, we mean disorders in one or more of the stomach, duodenum, jejunum plus ileum, and colon. Such disorders *e 2a 39 WO 91/12018 PCNrAU91/00031 -3may relate to intestinal diseases and/or surgical treatments. Thus where reference is made herein in general terms to the treatment of intestinal diseases, it is to be understood that we include the treatment of non-diseased intestines, part of which have been surgically removed and where increased growth of the residual intestine may be advantageous.

The term "peptide analogue", as used herein, includes one or more of the peptide analogues referred to in applicant's International Patent Applications PCT/AU86/00246 and PCT/AU88/00485, or fusion proteins deLived therefrom as described in International Patent Application PCT/AU90/00210, referred to above, the entire disclosures of which are incorporated herein by reference.

An effective amount of mammalian IGF-I or an analogue of IGF-I is defined as that needed to increase the weight of gut tissue by more than approximately above the weight of gut tissue prior to treatment.

Surprisingly IGF-I and its analogues have now been found by the applicants to increase the weight of the stomach, duodenum, jejunum plus ileum, and colon as well as the total gut weight. Of particular significance is the fact that these effects on growth have been found to occur in animals under a range of conditions, including in animals in which gut function had previously been markedly compromised by the surgical removal of a substantial portion of the jejunum plus ileum animals to which glucocorticoids have been administered in order to produce a catabolic state animals in which diabetes had been induced by the drug streptozotocin, a condition that led to gut growth so that the effects of IGF-I were above an already-stimulated growth state, and animals which had compromised kidney function.

Since glucocorticoids are administered to humans as a current treatment for the inflammation that characterizes several gut diseases, the present discovery that gut growth can be partially restored by IGF-I or its analogues even in the presence of glucocorticoids is both WO 91/12018 PCT/AU91/00031 -4surprising and advantageous.

In a preferred aspect of the present invention a peptide analogue to mammalian, preferably human, IGF-I is administered. Preferably the peptide analogue is an analogue wherein from 1 to 5 amino acid residues are absent from the N-terminal of mammalian IGF-I. Preferably 3 amino acid residues are absent therefrom. Such peptide analogue has been designated des(l-3)IGF-I.

Alternatively the peptide analogue may be an analogue wherein at least the glutamic acid residue is absent at position 3 from the N-termi.i al of mammalian IGF-I, and optionally replaced by a different amino acid residue. Preferably the analogue is one wherein the glutamic acid residue is replaced by an arginine residue.

More preferably the peptide analogue has an N-terminal sequence selected from Val-Leu-Cys- Arg-Leu-Cys- Gly-Leu-Cys- Gly-Thr-Leu-Cys- Gly-Pro-Arg-Thr-Leu-Cys- Gly-Pro-Gly-Arg-Leu-Cys- Gly-Pro-Gly-Gly-Leu-Cys- Gly-Pro-Gly-Thr-Leu-Cys- Gly-Pro-Gln-Thr-Leu-Cys- Gly-Pro-Lys-Thr-Leu-Cys- Gly-Pro-Leu-Thr-Leu-Cyswith the Cys residue shown being that normally at position 6 from the N-terminal.

In a further alternative aspect, the peptide analogue is a fusion protein including a first amino acid sequence including approximately the first 100 N-terminal amino acids of methionine porcine growth hormone, or a fragment thereof; and a second amino acid sequence of mammalian insulin-like growth factor-1, or an analogue thereof, joined to the C-terminal of the first amino acid sequence.

Preferably the first amino acid sequence includes WO 91/12018 P(7I/AU91/00031 approximately the first 46, more preferably the first 11, N-terminal amino acids of methionine porcine growth hormone, or fragment thereof.

The IGF-I analogues include des(l-3)IGF-I, specified in the co-owned International application PCT/AU86/00246, which specification is included herein by reference and had been shown to increase the growth of cultured cells at lower dose rates than required for IGF-I. In the development of the present invention, des (1-3)IGF-I has surprisingly been shown to show this increased potency in vivo, in the treatment of disorders in gut function, since lower concentrations of the analogue than of IGF-I itself produce comparable increases in the growth of gut tissue.

The IGF-I analogues also include a fusion protein MpGH(11)VN/R 3 IGF-I (abbreviated to LR3), specified as Example 13 in the co-owned International Application PCT/AU90/00210, which specification is included herein by reference, and had been shown to increase the growth of cultured cells at lower dose rates than required for IGF-I. In the present inventin, LR 3 has also surprisingly been shown to show increased potency in the treatment of disorders in qut function, since lower concentrations of the analogue than of IGF-I itself produce comparable increases in the growth of gut tissue.

Although the method in particular applies to the treatment of human subjects with IGF-I or an analogue of IGF-I, it can also be applied veterinarily to animals with intestinal diseases° Accordingly, in a further aspect, the present invention provides a pharmaceutical or veterinary composition for the treatment of disorders in gut function including: an effective amount of a mammalian, preferably human, IGF-I or peptide analogue thereof; and a pharmaceutically or veterinarily acceptable diluent, carrier or excipient therefor.

In a preferred form, the present invention vides a pharmaceutical or veterinary composition pro WO 91/12018 PCP/AU91/00031 -6wherein the IGF-I or the analogue of IGF-I is present in amounts sufficient to provide a dose rate of approximately to 2000, preferably 100 to 1000 micrograms/kg body weight/day.

In a further preferred aspect of the present invention, there is provided a method for the treatment of disorders in gut function which method includes administering to a patient to be treated a pharmaceutical or veterinary composition including an effective amount of a mammalian, preferably human, IGF-I or peptide analogue thereof, and a pharmaceutically or veterinarily acceptable diluent, carrier or excipient therefor; intravenously, subcutaneously, intramuscularly or enterally at a dose rate of approximately 10 to 2000, preferably 100 to 1000 micrograms/kg body weight/day.

Treatment may continue for a period of approximately 1 to days, preferably approximately 5 to 30 days.

The dose rate, dose intervals and treatment period may be adjusted to the degree of intestinal disease and the route of administration. Caution should be taken that blood glucose is monitored so that hypoglycemia can be prevented.

The dose rates and intervals for the administration of des(l-3)IGF-I and related analogues may be set at levels proportionally adjusted to the relative potency of the analogue to that of IGF-I itself. For example the levels for des(l-3)IGF-I or LR 3 will be proportionally less than for the full IGF-I peptide in accordance with the increased potency of des(l-3)IGF-I or

LR

3 Dose rates of 50 to 500 micrograms of des(l-3) IGF-I LR 3 /kg body weight/day are preferred.

In a still further aspect of the present invention there is provided the use of a mammalian insulin-like growth factor-1 (IGF-I) or a peptide analogue thereof for the manufacture of a pharmaceutical or veterinary preparation for the treatment of disorders in gut function.

The pharmaceutical or veterinary preparations may WO 91/12018 PCT/AU91/00031 -7be prepared utilising conventional techniques.

The benefits and parameters of the present.

invention will now be more fully described with reference to the accompanying examples. It should be understood, however, that the following description is illustrative only and should not be taken in any way as a restriction of the generality of the foregoing description.

EXAMPLE 1 Effects of IGF-I and des(1-3)IGF-I on stomach growth in the growth hormone-deficient lit/lit mouse At 6 weeks of age lit/lit mice were housed individually and weighed on a daily basis, and by 8 weeks of age it had been established that body growth had virtually ceased.

Mice were then randomised into 5 groups according to body weight and sex and were injected daily for 20 days with 120 pl of a sterile solution containing one part of HC1 (10 mmol/1) and nine parts of potassium phosphate (50 mmol/1), NaC1 (150 mmol/l) and 0.1% human serum albumin at pH 7.4 (diluent), 120 pl of diluent containing 3 pg IGF-I, 120 pl of diluent containing 3 pg des(l-3)IGF-I, 120 p1 of diluent containing 30 pg IGF-I, or 25 120 pl of diluent containing 30 pg des(l-3)IGF-I.

Each dose was administered subcutaneously as two injections, one at 9-10 am, the other at 4-5 pm. The animals were weighed and their lengths measured at 7 day intervals.

On day 21 the animals were killed by an anaesthetic overdose and tissues removed for weighing.

The body weights, animal lengths (including tail) and stomach weights are shown in the following Table 1.

Values are mans standard errors with statistical significance from diluent-treated control animals shown as *P<0.05; The numbers of animals are given in parentheses.

R. Since the initial body weights were 10 grams for each group, the daily dose rates were approximately WO 91/12018 PC/AU910031 -8equivalent to 300 pg and 3000 pg of each peptide per kg body weight.

Stomach weights, expressed as a percentage of the diluent group, were 105% and 123% with 300 pg and 3000 pg/kg body weight/day of IGF-I respectively, and 110% and 123% with 300 pg and 3000 pg/kg body weight/day of des(l-3)IGF-l respectively.

EXAMPLE 2 Effects of IGF-I and des(1-3)IGF-I LR 3 on out weights in dexamethasone-treated rats Male Hooded Wistar rats, weighing on average 152 g (range 138-164 g) and maintained in metabolism cages, had Alzet model 2001 osmotic pumps insert. subcutaneously within the scapular region under ether anaesthesia. One pump delivered dexamethasone at 20 micrograms/d and the other either 0.1M acetic acid as diluent; IGF-I at 111 pg/d; IGF-I at 278 pg/d; IGF-I at 695 pg/d; des(l-3) GF- at 44 pg/d; des(l-3)IGF-I at 111 pg/d; des(l-3)IGF-I at 278 pg/d;

LR

3 at 44 pg/d;

LR

3 at 11i1 pg/d;

LR

3 at 278 pg/d.

Animals were maintained in the metabolism cages for 7 days with daily measurements of body weight, food and nitrogen intake and nitrogen excretion. After this period the animals were killed by exsanguination under anaesthesia and the gastro-intestinal tract from stomach to colon was removed and separated into stomach, duodenum, jejunum plus ileum, cecum and colon. All regions were cleared of food or fecal contents and weighed.

The body weights and the weights of the different regions of the gastrointestinal tract are given as means standard errors in Table 2. Statistical significance from the diluent-treated group is shown as *P<0.05; There were six animals in each WO 91/12018 PC~/AU91/00031 -9group.

The weights of the total gut from stomach through colon is depicted in Figure 1 as a fraction of total body weight in the format of dose-response curves for IGF-I, des(l-3)IGF-I and LR 3 For a midpoint region of the ileum and the colon a portion was cut longitudinally and scraped to remove the mucosal layer. The weight of this layer was expressed as a percentage of the total mucosa plus muscularis. The protein contents of the same regions of the ileum were measured and expressed as mg per gram wet weight of tissue.

These values are given as means standard errors in Table 3. Statistical significance from the diluent-treated animals was not achieved using ANOVA (P>0.05).

This example demonstrates marked increases in the weights of different regions of the gut of dexamethasonetreated rats following the administration OF IGF-I, des(l-3)IGF-I or LR 3 The effects are dose dependent and are greater for des(l-3)IGF-I or LR 3 at doses equivalent to IGF-I.

The increased growth occurs predominantly through an expansion in the cross-sectional area of the gut because the length of each region is either not increased or increased only slightly.

It is evident from Figure 1 that the increase in gut weight is proportionally above that occurring for body weight.

Both mucosal and muscularis regions of the jejunum and colon show increased growth because the percent by weight accounted for by the mucoss is not affected by IGF treatment.

Growth occurs by an increase in tissue protein since the percent protein content of the jejunum and colon is not changed by IGF treatment.

EXAMPLE 3 Ouantitative histology of the duodenum from rats in Example 2 The mid region of the duodenum from certain animals in Example 1 was fixed in Bouin's fixative, WO 91/12018 PCZT/AU91/00031 dehydrated, embedded, transverse sections cut and stained with haematoxylin and eosin for quantitative histological analysis. All animals in groups and of Example 2 were processed and measurements of villus height, crypt depth, mucosal arer, submucosal area, muscularis externa area and total cross-sectional area were obtained. For each duodenum, 30 villus heights, crypt depths and 8 area measurements were averaged to obtain representative values. Means t SEM are shown in Table 4.

This example establishes that the growth of the duodenum produced by IGF-I, des(l-3)IGF-I or LR 3 at dose rates of 278 pg/d is accompanied by statistically significant (P<0.01) increases in cross-sectional area.

The increase is predominantly in the mucosal area, although the muscularis layer is also increased. The villi that make up much of the mocusa and play a key role in digestion and absorption, are also increased in height.

EXAMPLE 4 Effects of IGF-I and des(1-3)IGF-I on gut weights in rats treated following partial resection of the leiunum plus ileum Male Sprague Dawley rats, weighing on average 175 g (range 160-193 g) and maintained in metabolism cages, had Alzet model 2001 osmotic pumps inserted as in Example 2. The dose rages of growth factors were 170 pg/d for IGF-I and for des(l-3)IGF-I as well as a higher dose rate of 425 pg IGF-I/d. At the same time as the pum, were inserted subcutaneously, and using tribromethanol in amylene hydrate anaesthesia and aseptic techniques, the jejunum plus ileum was exposed through a mid-line incision. The mid 80% of these parts of the intestine was removed starting 10 cm from the ligament of Treitz and finishing 10 cm from the ileo-cecal valve. The intestine and abdominal cavity were bathed frequently in sterile saline containing penicillin (1000 U/ml). To further guard against possible infection, the animals were injected with 0.6 ml of procaine penicillin before surgery and again 4 days later. The animals were returned to WO 91/12018 PCIPAU91/00031 -11their metabolic cages and allowed free access to food and water. Body weights, food intakes, nitrogen intakes and nitrogen outputs were measured daily.

After 7 days of treatment, the animals were killed by exsanguination under anaesthesia and the gastro-intestinal tract from stomach to colon was removed and separated into stomach, duodenum, residual jejunum plus ileum, colon and cecum. All collected regions of the gut were cleared of food or fecal contents and weighed.

The body weights and the weights of the different regions of the gut are given as means standard errors in Table Statistical significance from the diluent-treated group is shown as *P<0.05; There were 7 animals in the diluent and des(l-3)IGF-I groups, six in the group with the low dose of IGF-I and five in the group with the high dose of IGF-I.

The example shows that des(l-3)IGF-I and a fold higher dose c IGF-I produce pronounced growth effects on the gut. A dose of IGF-I equal to that of des(l-3)IGF-I gave no statistically-significant effects.

The total gut weight less the residual jejunum and ileum, expressed as a percentage of the diluent group, was 113% with 170 pg IGF-I/d, 131% with 425 pg IGF-I/d, and 125% with 170 pg des(l-3)IGF-I/d.

EXAMPLE Effects of IGF-I, des(l-3)IGF-I and MpGH(11)VN/R 3

IGF-I

(LR

3 on aut growth in diabeti, rats Male Hooded-Wistar rats weighing approximately 150 g were injecte( with streptozotocin intra-peritoneally at a dose of 70 mg/kg and transferred to metabolic cages.

Diabetes was confirmed by blood gucose measurements.

After 7 days (average body weight 162 g) the animals were implanted with osmotic pumps in exactly the same way and to deliver exactly the same doses as in Example 1. After 7 days treatment the animals were killed and the weights of the following gut organs measured: stomach, duodenum, ileum plus jejunum and colon. These values are shown in Table 6 and the total gut weights in Figure 2. Each value WO 91/12018 Pk-,/AU91/00031 -12is the mean SEM for six animals. Statistical significance (ANOVA; least significant difference) is shown by *P<0.05, ***P<0.001 versus diluent-treated diabetic rats.

These results demonstrate that IGF-I and lower doses of des(1-3)IGF-I or LR 3 produce substantial growth effects on the stomach, ileum plus jejunum, colon and total gut weights. Effects: on the duodenum are somewhat less.

The response of IGFs in the diabetic rats is especially important since even untreated animals already have heavier gut weights as a result of the hyperphagia associated with this condition. For example the weight of ileum plus jejunum was 5.08±0.29 g in another group of animals in which the diabetes was treated by insulin administration. This is lower than the diluent group in Table 5 notwithstanding the fact that the body weight of the insulin-treated animals was much heavier (231±8g).

EXAMPLE 6 Effects of IGF-I and des(l-3)IGF-I on qut 'Teights in rats followina partial nephrectomv Partial renal failure was produced in Sprague Dawley male rats (95-125 g) by a 2-stage sub-total nephrectomy. This was performed via flank insicions, by ligating terminal branches of the left renal artery to give ischemia of at least half of the left kidney (Day 0), with a right nephrectomy being undertaken one week later, at which time the right jugular vein was also cannulated (Day Partially nephrectomized rats were selected on day 14 for inclusion in the treatment period of the study on the basis of detectable proteinuria, and of increased urine volume and serum urea levels at least twoce those of the sham-operated control animals. On Day 16 treatment was commenced by means of mini-osmotic pumps (Alzet Model 2001, Alza Co., Palo Alto, California) which were implanted subcutaneously in the dorsal thoracic region under halothane anesthesia. Nephrectomized rats were randomly allocated to 4 treatment groups: diluent treated 0.1M acetic acid), low dose IGF-I treated (170 yg/d), WO 91/12018 PCF1/AU91/00031 -13high dose IGF-I treated (425 pg/d), or des(1-3)IGF-I treated (170 pg/d). The average body weight at time of pump insertion was 193 g. Animals were killed on Day 23 and gut weights measured as in Example 2. These are shown in Table 7. Statistical significance from diluent-treated animals is indicated by *P<0.05, **P<0.01.

This example demonstrates that gut weights are increased by 7 days treatment with IGF-I or des(l-3)IGF-I in rats that are compromised by partial nephrectomy.

Finally, it is to be understood that various other modifications and/or alterations may be made without departing from the spirit of the present invention as outlined herein.

TABLE 1 Growth effect2 of IGF-I and des(1-3)IGF-I over a 20-day treatment period of lit/lit mice Treatment Group Body Animal Stomach Weight Length (mm) Weight (mg) Diluent 10.20±0.19 124±2 64.3±3.0 IGF-I, 3 pg/d 10.75±0.28 127±1 67.8±2.1 jg/d 11.25±0O.41 132±1* 79.0±3.0** des(1-3)GF-I, 3 pg/d 10.76±0.31 127±2 70.6t2.5 pg/d 11.33±0.42 132±1 79.3±4.4** TABLE 2 Gut weights lengths (cm) and body weights of dexamethasone-treaated Eats, also treated with IGF-I. des(I-3)IGF-I or LR 3 Body Stomach Duodenum Treatment Weight Weight Weight Length Diluent 131t3 0.87±0.03 0.50t0.02 7.2±0.4 IGE'-I, 111 pg/d 130±4 0.93±0.03* 0.55±0.03 6.9±0.3 2 78 ijl d 143:A* 1.09t0.O2*** 0.70t0.02*** 7.6±0.2 695 pg/d 158±2*** 1.17±0.02*** 0.84±0.02*** 8.0±0.2* des(1-3)IGF-1, 44 pig/d 135±3 0.98±0.02** 0.63±0.03** 7.6±0.3 111 pig/d 1.44±~5* 1.06±0.02*** 0.68±0O.02*** 7.6±0.2 2718 pig/d 151±2*** 0.86±0.03*** LR 3 44 pg/d 135±1 0.95±0.01* 0.61±0.02** 7.3±0O.3 111 ,-tg/d 140±4 1.07±0.02*** 0.75t0.03*** ".6±0.4 278 1 igld 150±3*** 1.16-0.02*** 0.86±0.03*** 8.3±0.2** TABLE 2 CONTINUED Illeum Jejunum Colon Weight Length Weight Length 3 .070. .22 3. .60±0. 19 4.30±0.21* .22±0.23*** 3. 80±0 .25* 4.44±0.24* 5.09±0. 21*** 3 .93±0O.24** 4.67±0.18* 5.20±0.33* 70.8-4.1 7 1.8±t2. 6 7 1.7±L3. 1 86. 1±3 6 72. 1±3. 5 71. 8±2. 6 73 .0±4 1 72 8 75. 8t3 .3 79. 5±4. 1 0. 68±0 05 0. 64±0. 02 0.92±0.04* 0.93±0.05* 0. 72±0. 05 0.86±0. Q4** 0. 91±0.04*** 0. 75±0. 03 0.89±0. 05** 0.98±0.05* 11. 0±0. 4 12. 0±0. 3 13.3±0. 6 12 7±0O. 6 11. 3±0. 8 13 4±0O 11. .3±0 8 12. 3±0. 2 12 5±0 8 12. 9±0. 6 TABLE 3 Fractional weights and Protein contents of the ieiunum in the mucosal layers in the jejunum and in the colon dexamethasone-treated rats treated with IGFS Jei unum Colon Treatment Mucosa Mucosa Muscularis Mucosa of total) ProtCein Protein of total) (mg/g weight) (mg/g weight) Di luent 55.1±3.3 124±5 169±t4 30.5±2.5 IGF-I, 111 pgfd 58.8±2.2 117±6 151t4 29.6±1.7 278 jg/d 62.7±1.5 135±5 161±5 31.7±1.7 695 pg/d 61.1±2.8 136±t5 159±2 28.8±1l.2 des(I-3)IGF-I, 44 pg/d 53.3±3.9 134±5 161±5 31.1±1.7 111 jgfd 59.6±2.3 140±5 162±4 271.5±2.2 278 pg/d 55 .3±3 .6 140±4 154±6 32.5±2.5 LR 3 44 pg/cl 56.8±4.2 119±10 147±4 30.2±2.8 I11l pg/cl 60 .7±3 .3 139±4 168±6 29.6±2.1 278 pg/cl 54.2±3.2 135±6 159±:5 30.6±2.2 TABLE 4 Sections from rats treated with IGF-I des(1-3)IGF-I. LR 3or diluent Treatment Group Measurement Diluent IGF-I des(1-3)IGF-I LR 3 Villus height (mm) 0.65±0.02 0.76±0.03 0.73±0,03 0.84±0.03*** Crypt depth (mm) 0.20±0.01 0.23±0.01 0.23±0.00 0.23±0.01 Villus :crypt ratio 3.3 ±0.2 3.4 ±0.2 3.3 ±0.1 3.7 ±0.2 Mucosal area (mm 2) 5.67±0.44 7.72±0.56** 8.03±0.58** 8.29±0.56*** Sub-mucosal area (mm 2 0.42±0.04 0.51±0.04 0.52±0.03 0.51±0,04 Musc. externa area (mm 2 1.20±0.15 1.51±0.05* 1.54±0.06** 1.41±0.12 Total area (mm 2) 7.29±0.61 9.74±0*59** 10.10±0.62** 10.21±0.66** *P<0.05, **P<Qo]1 ***P<0.001 versus diluent TABLE Diluent IGF-I IGF-I des(1-3)IGF-1 Duodenum weight (mg) 170 1 .g/d 425 pg/d 170 pg/d Body weight (g) Stomach weight (mg) Duodenum weight (mug) 171. u 4. 4.5 980 75 1067 1984 4- 118 1067 ±162 4 .28 ±0.27 173.4 9 1089 4± 47 1179 88 2217 244 1305 ±164 4.83 ±0.34 1236* 4- 26 1572** ±81 190.9 ±4.2 184 .1 4- 5.6 113 6* ±52 1542* +102 Residual Jejunum ileum weight (mug) Colon weight (g) Total gut weight less residual jejunumn ileum (g) 2288 60 1330 ±65 2259 150 1250 127 5. 59** ±0.13 5. 37** ±0.24 TABLE 6 Gut weigihts (ci) of diabetic rats and body weights Body Stomach Duodenum Ileum Colon Weight Jej unum Diluent, 172±6 1.01±0.04 0.72±0.09 6.10±0.49 0.95±0.02 IGF-I, 111 pg/d 186±4 1.13±0.04 0.74±0.08 6.21±0.37 1.05±0.07 278 pg/d 198±8s* 1.19±0.06* 0.91±0.05 7.41±0.32* 1.09±0.05 695 pg/d 210±8*** 1.44±0.08*** 0.94±0.06* 8.17±0.32*** 1.18±0.05** des(1-3)IGF-I, 44 pig/d 185±6 1.23±0.05** 0.82±0.11 6.83±0.38 1.02±0.05 111 pg/d 194±7* 1.27±0.06** 0.89±0.07 7.97±0O.20** 1.16.0.08"* 278 pg/d 212±8*** 1.49±0.07*** 1.02±0.09** 8.69±0.40*** l.41±0.03*** LR 3 44 pig/d 1 -0±7 1.14±0.06 0.85±0.07 7.58±0O.48* 1.05±0,04 il1. p~g/d 204±6** 1.38±0.04*** 0.88±0.11 7.83±0.53** 1.25±0.07*** 278 pg/d 213±8*** 1.48±0.08*** 0.91±0.06 8.47±0.46*** 1.50±0.04*** TABLE 7 Gut weights in partiallv'-nephrectomised rats treated with IGF-I or des(1-3)IGF-IE Treatment Stomach Duodenum Ileum Colon Tota'- Jej unum Di luent IGF-I, 170 pg/d 425 pg/d des(1-3)IGF-I 170 pigfd 1.08±0.04 1. 19±0. 03 1. 25±0.06* 1. 16±0. 06 0.51.0. 02 0. 63±0.03* 0.75±0O.07** 0.66±0.03* 3. 78±0. 19 4.70±0.27** 5.11±0. 22** 4.48±0.15* 0 83±0 03 0.97±0.03* 1.05±0. Q7** 0 95±0 06 6.21±0. 22 7.50±0.30** 8.16±0. 27** 7.24±0.10**

Claims

1. A method for the treatment of disorders in gut function in animals including humans, which method includes administering to a patient to be treated an effective amount of a mammalian insulin-like growth factor-I (IGF-I) or a peptide analogue thereof.

2. A method according to Claim 1 wherein the IGF-I or peptide analogue thereof is administered in an amount of from approximately 10 to 5000 microgram/kg body weight/day for a period of approximately 1 to 60 days.

3. A method according to Claim 1, which method includes administering to a patient an effective amount of human insulin-like growth factor-I.

4. A method according to Claim 1, which method includes administering to a patient an effective amount of a peptide analogue of mammalian insulin-like growth factor-I, wherein from 1 to 5 amino acid residues are absent from the N-terminal thereof.

A method according to Claim 3, wherein 3 amino acid residues are absent from the N-terminal thereof.

6. A method according to Claim 4, wherein the peptide analogue is administered at a dose rate of approximately 50 to 500 micrograms/kg body weight/day for a period of approximately 1 to 60 days.

7. A method according to Claim 1, which method includes administering to the patient an effective amount of a peptide analogue of mammalian insulin-like growth factor-I, wherein at least the glutamic acid residue is absent at position 3 from the N-terminal thereof, and is optionally replaced by a different amino acid residue.

8. A method according to Claim 7, wherein the glutamic acid residue is replaced by an argenine residue.

9. A method according to Claim 7, wherein the peptide analogue has an N-terminal sequence selected from Val-Leu-Cys- Arg-Leu-Cys- Gly-Leu-Cys- Gly-Thr-Leu-Cys- Gly-Pro-Arg-Thr-Leu-Cys- Gly-Pr -Gly-Arg-Leu-Cys- WO 91/12,18 PCrT/AU91/00031 -23- Gly-Pro-Gly-Gly-Leu-Cys- Gly-Pro-Gly-Thr-Leu-Cys- Gly-Pro-Gln-Thr-Leu--Cys- Gly-Pro-Lys-Thr-Leu-Cys- Gly-Pro-Leu-Thr-Leu-Cys- with the Cys residue shown being that normally at position 6 from the N-terminal.

A method according to Claim 6 wherein the peptide analogue is administered at a dose rate of approximately 50 to 500 micrograms/kg body weight/day for a period of approximately 1 to 4 days.

11. A method according to Claim 1, which method includes administering to a patient an effective amount of a peptide analogue of mammalian insulin-like growth factor-I which is a fusion protein including a first amino acid sequence including approximately the first 100 N-terminal amino acids of methionine porcine growth hormone, or a fragment thereof; and a second amino acid sequence of mammalian insulin-like growth factor-I, or an analogue thereof, joined to the C-terminal of the first amino acid sequence.

12. A method according to Claim 10, wherein the first amino acid sequence includes approximately the first 46, more preferably the first 1 N-terminal amino acids of methionine porcine growth hormone, or fragment thereof.

13. A method according to Claim 10, wherein the peptide analogue is administered at a dose rate of approximately 50 to 500 microgram/kg body weight/day for a period of approximately 1 to 60 days.

14. A pharmaceutical or veterinary composition, for the treatment of disorders in gut function, including an effective amount of a mammalian insulin-like growth factor-I or peptide analogue thereof; and a pharmaceutically or veterinarily acceptable diluent carrier or excipient therefor.

A pharmaceutical or veterinary composition according to Claim 14, wherein the insulin-like growth i) factor-I or analogue thereof is present in amounts WO 91/12018 PCT/AU91/00031 -24- sufficient to provide a dose rate of approximately 10 to 5000 microgram/kg body weight/day.

16. A method for the treatment of disorders in gut function, which method includes administering to a patient to be treated a pharmaceutical or veterinary composition including an effective amount of a mammalian insulin-like growth factor-I or analogue thereof; and a pharmaceutically or veterinarily acceptable .0 diluent carrier or excipient therefor intravenously, subcutaneously, intramuscularly or enterily at a dose rate of approximately 10 to 5000 microgram/kg body weight/day for a period of approximately 1 to 60 days.

17. A method of manufacturing a pharmaceutical or veterinary preparation for treating disordp-s in gut Cunction comprising adding a mammalian insulin-like growth facto:-l (1GF-1) or a peptide analogue thereof to a pharmaceutically or veterinarily acceptable diluent carrier or excipient therefor.

18. A method according to Claim 1 ;ubstantially as hereinbefore described with reference to any one of the Examples. DATED: 4 March, 1993 PHILLIPS ORMONDE FITZPATRICK Attorneys for: GROPEP PTY. LTD. fi;: r v 4 a a a. a. a. S